Described herein are methods of screening one of the RNA hairpins in the small ribosomal subunit of bacteria to identify peptides that bind to it. The RNA hairpin target may be the 970 loop (aka helix 31 (h31)) or a modified version thereof. The identified peptides may inhibit protein synthesis and, therefore, may be used as a model for new antibiotics.
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This application claims the benefit of priority to U.S. Provisional Patent Application Ser. No. 61/151,412, filed Feb. 10, 2009, which is hereby incorporated by reference in its entirety.
The increasing emergence of antibiotic resistant bacteria is a global problem. [Fauci, A. S., Touchette, N. A. & Folkers, G. K. (2005). Emerging infectious diseases: a 10-year perspective from the national institute of allergy and infectious diseases. Emerg Infect Dis 11, 519-25.] Antibiotic resistant bacteria were responsible for 17 million deaths world-wide in 1996 with an estimated cost of $30 billion dollars in the United States alone. [Levy, S. B. & Marshall, B. (2004). Antibacterial resistance worldwide: causes, challenges and responses. Nat Med 10, S122-9.] Funding for new research by major pharmaceutical companies has steadily decreased, as has the development of new antimicrobials. Furthermore, the rapid emergence of resistance to new classes of antimicrobials has limited their use in clinical settings. These trends, if continued, will result in a lack of effective antimicrobials for a majority of bacterial infections in the years to come.
The mechanism of resistance for all currently-used therapeutics has been determined. There are several general mechanisms of bacterial resistance: 1) reduction of antibiotic uptake, 2) transport of the antibiotic out of the cell, 3) enzymatic inactivation of the antibiotic, 4) use of an alternative metabolic pathway, 5) titration of the antibiotic by overproduction of the target, and 6) target modification so that it is no longer recognized by the antibiotic. [Laios, E., Waddington, M., Saraiya, A. A., Baker, K. A., O'Connor, E., Pamarathy, D. & Cunningham, P. R. (2004). Combinatorial genetic technology for the development of new anti-infectives. Arch Pathol Lab Med 128, 1351-9.] Of these mechanisms, target modification is the most common mechanism of resistance for newly-developed antibiotics. The specificity of antibiotic-target binding involves the structure as well as the sequence of the target. Mutations that affect the sequence or structure of the target without affecting function may reduce or eliminate antibiotic binding and result in resistance. For example, aminoglycoside antibiotics target the A-site of bacterial 16 S ribosomal RNA and increase the translational error rate. [Magnet, S. & Blanchard, J. S. (2005). Molecular insights into aminoglycoside action and resistance. Chem Rev 105, 477-98.] A single A1408G mutation reduces ribosome function by approximately 30% but completely disrupts binding of certain aminoglycoside antibiotics. [Recht, M. I., Douthwaite, S., Dahlquist, K. D. & Puglisi, J. D. (1999). Effect of mutations in the A site of 16 S rRNA on aminoglycoside antibiotic-ribosome interaction. J Mol Biol 286, 33-43.] Therefore, targeting an antibiotic to all possible mutants of a particular ribosomal region that maintain function would eliminate this mechanism of resistance.
Nearly half of all naturally-occurring antibiotics target an aspect of protein synthesis and more specifically the ribosome. The 70 S bacterial ribosome is responsible for the translation of messenger RNA (mRNA) into protein. Ribosome crystal structures and biochemical studies have shown that the RNA is the catalytically-active component of the ribosome, therefore, the ribosome is a ribozyme. [Yusupov, M. M., Yusupova, G. Z., Baucom, A., Lieberman, K., Earnest, T. N., Cate, J. H. & Noller, H. F. (2001). Crystal structure of the ribosome at 5.5 A resolution. Science 292, 883-96; Wimberly, B. T., Brodersen, D. E., Clemons, W. M., Jr., Morgan-Warren, R. J., Carter, A. P., Vonrhein, C., Hartsch, T. & Ramakrishnan, V. (2000). Structure of the 30S ribosomal subunit. Nature 407, 327-39.] The essential nature of the protein synthesis process makes the ribosomal RNA (rRNA) an ideal drug target.
Studies of the rRNA sequences from numerous different organisms have shown that the overall structure of the ribosome is conserved within all three domains of life. Phylogenetic analysis of rRNA sequences has provided much information about pairing interactions and nucleotide conservation. Each of these analyses, however, employs genomic or organelle rRNA sequences. These sequences are constrained by their essential role in protein synthesis. As a result, very little or no sequence variation is observed in rRNA regions believed to be functionally important, since even subtle changes to the structure surrounding critical residues may reduce function and affect fidelity. Additionally, these conserved sites may be structurally important rather than functionally important. Therefore, drugs that target these sites would allow for resistance if the sequence can mutate but maintain the functional structure. An ideal drug would target all possible functional mutations at the target site.
In certain embodiments, the invention relates to screening one of the RNA hairpins in the small ribosomal subunit of bacteria to identify peptides that bind to it and therefore have the potential to serve as leads for further development into antibiotics.
In certain embodiments, the invention relates to the peptides so identified.
In certain other embodiments, the invention relates to the use of the RNA hairpin, 970 loop aka helix 31 (h31), as a target, and the peptides identified herein.
In certain further embodiments, the invention relates to derivatives of the identified peptides.
In certain other embodiments, the invention relates to peptides that inhibit protein synthesis.
In certain other embodiments, the invention relates to methods of using the peptides to create new antibiotics.
The articles “a” and “an” are used herein to refer to one or more than one (i.e., to at least one) of the grammatical object of the article.
The term “amino acid” is known in the art. In general the abbreviations used herein for designating the amino acids and the protective groups are based on recommendations of the IUPAC-IUB Commission on Biochemical Nomenclature (see Biochemistry (1972) 11:1726-1732). In certain embodiments, the amino acids used in the application of this invention are those naturally occurring amino acids found in proteins, or the naturally occurring anabolic or catabolic products of such amino acids which contain amino and carboxyl groups. Particularly suitable amino acid side chains include side chains selected from those of the following amino acids: glycine, alanine, valine, cysteine, leucine, isoleucine, serine, threonine, methionine, glutamic acid, aspartic acid, glutamine, asparagine, lysine, arginine, proline, histidine, phenylalanine, tyrosine, and tryptophan.
The term “amino acid” further includes analogs, derivatives and congeners of any specific amino acid referred to herein, as well as C-terminal or N-terminal protected amino acid derivatives (e.g. modified with an N-terminal or C-terminal protecting group). For example, the present invention contemplates the use of amino acid analogs wherein a side chain is lengthened or shortened while still providing a carboxyl, amino or other reactive precursor functional group for cyclization, as well as amino acid analogs having variant side chains with appropriate functional groups). For instance, the subject compound can include an amino acid analog such as, for example, cyanoalanine, canavanine, djenkolic acid, norleucine, 3-phosphoserine, homoserine, dihydroxy-phenylalanine, 5-hydroxytryptophan, 1-methylhistidine, 3-methylhistidine, diaminopimelic acid, ornithine, or diaminobutyric acid. Other naturally occurring amino acid metabolites or precursors having side chains which are suitable herein will be recognized by those skilled in the art and are included in the scope of the present invention.
Also included are the (d) and (l) stereoisomers of such amino acids when the structure of the amino acid admits of stereoisomeric forms. The configuration of the amino acids and amino acid residues herein are designated by the appropriate symbols (d), (l) or (dl), furthermore when the configuration is not designated the amino acid or residue can have the configuration (d), (l) or (dl). It will be noted that the structure of some of the compounds of this invention includes asymmetric carbon atoms. It is to be understood accordingly that the isomers arising from such asymmetry are included within the scope of this invention. Such isomers can be obtained in substantially pure form by classical separation techniques and by sterically controlled synthesis. For the purposes of this application, unless expressly noted to the contrary, a named amino acid shall be construed to include both the (d) or (l) stereoisomers. D- and L-α-Amino acids are represented by the following Fischer projections and wedge-and-dash drawings. In the majority of cases, D- and L-amino acids have R- and S-absolute configurations, respectively.
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In certain embodiments, polypeptides of the invention may be synthesized chemically, ribosomally in a cell free system, or ribosomally within a cell. Chemical synthesis of polypeptides of the invention may be carried out using a variety of art recognized methods, including stepwise solid phase synthesis, semi-synthesis through the conformationally-assisted re-ligation of peptide fragments, enzymatic ligation of cloned or synthetic peptide segments, and chemical ligation. Native chemical ligation employs a chemoselective reaction of two unprotected peptide segments to produce a transient thioester-linked intermediate. The transient thioester-linked intermediate then spontaneously undergoes a rearrangement to provide the full length ligation product having a native peptide bond at the ligation site. Full length ligation products are chemically identical to proteins produced by cell free synthesis. Full length ligation products may be refolded and/or oxidized, as allowed, to form native disulfide-containing protein molecules. (see e.g., U.S. Pat. Nos. 6,184,344 and 6,174,530; and T. W. Muir et al., Curr. Opin. Biotech. (1993): vol. 4, p 420; M. Miller, et al., Science (1989): vol. 246, p 1149; A. Wlodawer, et al., Science (1989): vol. 245, p 616; L. H. Huang, et al., Biochemistry (1991): vol. 30, p 7402; M. Schnolzer, et al., Int. J. Pept. Prot. Res. (1992): vol. 40, p 180-193; K. Rajarathnam, et al., Science (1994): vol. 264, p 90; R. E. Offord, “Chemical Approaches to Protein Engineering”, in Protein Design and the Development of New therapeutics and Vaccines, J. B. Hook, G. Poste, Eds., (Plenum Press, New York, 1990) pp. 253-282; C. J. A. Wallace, et al., J. Biol. Chem. (1992): vol. 267, p 3852; L. Abrahmsen, et al., Biochemistry (1991): vol. 30, p 4151; T. K. Chang, et al., Proc. Natl. Acad. Sci. USA (1994) 91: 12544-12548; M. Schnlzer, et al., Science (1992): vol., 3256, p 221; and K. Akaji, et al., Chem. Pharm. Bull. (Tokyo) (1985) 33: 184).
Certain compounds of the present invention may exist in particular geometric or stereoisomeric forms. The present invention contemplates all such compounds, including cis- and trans-isomers, R- and S-enantiomers, diastereomers, (d)-isomers, (l)-isomers, the racemic mixtures thereof, and other mixtures thereof, as falling within the scope of the invention. Additional asymmetric carbon atoms may be present in a substituent such as an alkyl group. All such isomers, as well as mixtures thereof, are intended to be included in this invention.
If, for instance, a particular enantiomer of a compound of the present invention is desired, it may be prepared by asymmetric synthesis, or by derivation with a chiral auxiliary, where the resulting diastereomeric mixture is separated and the auxiliary group cleaved to provide the pure desired enantiomers. Alternatively, where the molecule contains a basic functional group, such as amino, or an acidic functional group, such as carboxyl, diastereomeric salts are formed with an appropriate optically-active acid or base, followed by resolution of the diastereomers thus formed by fractional crystallization or chromatographic means well known in the art, and subsequent recovery of the pure enantiomers.
The term “conservative substitutions” refers to changes between amino acids of broadly similar molecular properties. For example, interchanges within the aliphatic group alanine, valine, leucine and isoleucine can be considered as conservative. Sometimes substitution of glycine for one of these can also be considered conservative. Other conservative interchanges include those within the aliphatic group aspartate and glutamate; within the amide group asparagine and glutamine; within the hydroxyl group serine and threonine; within the aromatic group phenylalanine, tyrosine and tryptophan; within the basic group lysine, arginine and histidine; and within the sulfur-containing group methionine and cysteine. Sometimes substitution within the group methionine and leucine can also be considered conservative. Preferred conservative substitution groups are aspartate/glutamate; asparagine/glutamine; valine/leucine/isoleucine; alanine/valine; valine/leucine/isoleucine/methionine; phenylalanine/tyrosine; phenylalanine/tyrosine/tryptophan; lysine/arginine; and histidine/lysine/arginine.
“Equivalent” when used to describe nucleic acids or nucleotide sequences refers to nucleotide sequences encoding functionally equivalent polypeptides. Equivalent nucleotide sequences will include sequences that differ by one or more nucleotide substitution, addition or deletion, such as an allelic variant; and will, therefore, include sequences that differ due to the degeneracy of the genetic code. For example, nucleic acid variants may include those produced by nucleotide substitutions, deletions, or additions. The substitutions, deletions, or additions may involve one or more nucleotides. The variants may be altered in coding regions, non-coding regions, or both. Alterations in the coding regions may produce conservative or non-conservative amino acid substitutions, deletions or additions.
“Homology” or alternatively “identity” refers to sequence similarity between two peptides or between two nucleic acid molecules. Homology may be determined by comparing a position in each sequence, which may be aligned for purposes of comparison. When a position in the compared sequence is occupied by the same base or amino acid, then the molecules are homologous at that position. A degree of homology between sequences is a function of the number of matching or homologous positions shared by the sequences.
The term “percent identical” refers to sequence identity between two amino acid sequences or between two nucleotide sequences. Identity may be determined by comparing a position in each sequence, which may be aligned for purposes of comparison. When an equivalent position in the compared sequences is occupied by the same base or amino acid, then the molecules are identical at that position; when the equivalent site is occupied by the same or a similar amino acid residue (e.g., similar in steric and/or electronic nature), then the molecules may be referred to as homologous (similar) at that position. Expression as a percentage of homology, similarity, or identity refers to a function of the number of identical or similar amino acids at positions shared by the compared sequences. Various alignment algorithms and/or programs may be used, including FASTA, BLAST, or ENTREZ. FASTA and BLAST are available as a part of the GCG sequence analysis package (University of Wisconsin, Madison, Wis.), and may be used with, e.g., default settings. ENTREZ is available through the National Center for Biotechnology Information, National Library of Medicine, National Institutes of Health, Bethesda, Md. In one embodiment, the percent identity of two sequences may be determined by the GCG program with a gap weight of 1, e.g., each amino acid gap is weighted as if it were a single amino acid or nucleotide mismatch between the two sequences. Other techniques for alignment are described in Methods in Enzymology, vol. 266: Computer Methods for Macromolecular Sequence Analysis (1996), ed. Doolittle, Academic Press, Inc., a division of Harcourt Brace & Co., San Diego, Calif., USA. Preferably, an alignment program that permits gaps in the sequence is utilized to align the sequences. The Smith-Waterman is one type of algorithm that permits gaps in sequence alignments. See Meth. Mol. Biol. 70: 173-187 (1997). Also, the GAP program using the Needleman and Wunsch alignment method may be utilized to align sequences. An alternative search strategy uses MPSRCH software, which runs on a MASPAR computer. MPSRCH uses a Smith-Waterman algorithm to score sequences on a massively parallel computer. This approach improves the ability to pick up distantly related matches, and is especially tolerant of small gaps and nucleotide sequence errors. Nucleic acid-encoded amino acid sequences may be used to search both protein and DNA databases. Databases with individual sequences are described in Methods in Enzymology, ed. Doolittle, supra. Databases include Genbank, EMBL, and DNA Database of Japan (DDBJ).
The terms “polynucleotide”, and “nucleic acid” are used interchangeably to refer to a polymeric form of nucleotides of any length, either deoxyribonucleotides or ribonucleotides, or analogs thereof. The following are non-limiting examples of polynucleotides: coding or non-coding regions of a gene or gene fragment, loci (locus) defined from linkage analysis, exons, introns, messenger RNA (mRNA), transfer RNA, ribosomal RNA, ribozymes, cDNA, recombinant polynucleotides, branched polynucleotides, plasmids, vectors, isolated DNA of any sequence, isolated RNA of any sequence, nucleic acid probes, and primers. A polynucleotide may comprise modified nucleotides, such as methylated nucleotides and nucleotide analogs. If present, modifications to the nucleotide structure may be imparted before or after assembly of the polymer. The sequence of nucleotides may be interrupted by non-nucleotide components. A polynucleotide may be further modified after polymerization, such as by conjugation with a labeling component. The term “recombinant” polynucleotide means a polynucleotide of genomic, cDNA, semi-synthetic, or synthetic origin, which either does not occur in nature or is linked to another polynucleotide in a non-natural arrangement. An “oligonucleotide” refers to a single stranded polynucleotide having less than about 100 nucleotides, less than about, e.g., 75, 50, 25, or 10 nucleotides.
The terms “polypeptide”, “peptide” and “protein” (if single chain) are used interchangeably herein to refer to polymers of amino acids. The polymer may be linear or branched, it may comprise modified amino acids, and it may be interrupted by non-amino acids. The terms also encompass an amino acid polymer that has been modified; for example, disulfide bond formation, glycosylation, lipidation, acetylation, phosphorylation, or any other manipulation, such as conjugation with a labeling component. As used herein the term “amino acid” refers to either natural and/or unnatural or synthetic amino acids, including glycine and both the D or L optical isomers, and amino acid analogs and peptidomimetics.
The term “specifically hybridizes” refers to detectable and specific nucleic acid binding. Polynucleotides, oligonucleotides and nucleic acids of the invention selectively hybridize to nucleic acid strands under hybridization and wash conditions that minimize appreciable amounts of detectable binding to nonspecific nucleic acids. Stringent conditions may be used to achieve selective hybridization conditions as known in the art and discussed herein. Generally, the nucleic acid sequence homology between the polynucleotides, oligonucleotides, and nucleic acids of the invention and a nucleic acid sequence of interest will be at least 30%, 40%, 50%, 60%, 70%, 80%, 85%, 90%, 95%, 98%, 99%, or more. In certain instances, hybridization and washing conditions are performed under stringent conditions according to conventional hybridization procedures and as described further herein.
The terms “stringent conditions” or “stringent hybridization conditions” refer to conditions, which promote specific hybridization between two complementary polynucleotide strands so as to form a duplex. Stringent conditions may be selected to be about 5° C. lower than the thermal melting point (Tm) for a given polynucleotide duplex at a defined ionic strength and pH. The length of the complementary polynucleotide strands and their GC content will determine the Tm of the duplex, and thus the hybridization conditions necessary for obtaining a desired specificity of hybridization. The Tm is the temperature (under defined ionic strength and pH) at which 50% of a polynucleotide sequence hybridizes to a perfectly matched complementary strand. In certain cases it may be desirable to increase the stringency of the hybridization conditions to be about equal to the Tm for a particular duplex.
A variety of techniques for estimating the Tm are available. Typically, G-C base pairs in a duplex are estimated to contribute about 3° C. to the Tm, while A-T base pairs are estimated to contribute about 2° C., up to a theoretical maximum of about 80-100° C. However, more sophisticated models of Tm are available in which G-C stacking interactions, solvent effects, the desired assay temperature and the like are taken into account. For example, probes can be designed to have a dissociation temperature (Td) of approximately 60° C., using the formula: Td=(((((3×#GC)+(2×#AT))×37)−562)/#bp)−5; where #GC, #AT, and #bp are the number of guanine-cytosine base pairs, the number of adenine-thymine base pairs, and the number of total base pairs, respectively, involved in the formation of the duplex.
Hybridization may be carried out in 5×SSC, 4×SSC, 3×SSC, 2×SSC, 1×SSC or 0.2×SSC for at least about 1 hour, 2 hours, 5 hours, 12 hours, or 24 hours. The temperature of the hybridization may be increased to adjust the stringency of the reaction, for example, from about 25° C. (room temperature), to about 45° C., 50° C., 55° C., 60° C., or 65° C. The hybridization reaction may also include another agent affecting the stringency, for example, hybridization conducted in the presence of 50% formamide increases the stringency of hybridization at a defined temperature.
The hybridization reaction may be followed by a single wash step, or two or more wash steps, which may be at the same or a different salinity and temperature. For example, the temperature of the wash may be increased to adjust the stringency from about 25° C. (room temperature), to about 45° C., 50° C., 55° C., 60° C., 65° C., or higher. The wash step may be conducted in the presence of a detergent, e.g., 0.1 or 0.2% SDS. For example, hybridization may be followed by two wash steps at 65° C. each for about 20 minutes in 2×SSC, 0.1% SDS, and optionally two additional wash steps at 65° C. each for about 20 minutes in 0.2×SSC, 0.1% SDS.
Exemplary stringent hybridization conditions include overnight hybridization at 65° C. in a solution comprising, or consisting of, 50% formamide, 10×Denhardt (0.2% Ficoll, 0.2% Polyvinylpyrrolidone, 0.2% bovine serum albumin) and 200 μg/ml of denatured carrier DNA, e.g., sheared salmon sperm DNA, followed by two wash steps at 65° C. each for about 20 minutes in 2×SSC, 0.1% SDS, and two wash steps at 65° C. each for about 20 minutes in 0.2×SSC, 0.1% SDS.
Hybridization may consist of hybridizing two nucleic acids in solution, or a nucleic acid in solution to a nucleic acid attached to a solid support, e.g., a filter. When one nucleic acid is on a solid support, a prehybridization step may be conducted prior to hybridization. Prehybridization may be carried out for at least about 1 hour, 3 hours or 10 hours in the same solution and at the same temperature as the hybridization solution (without the complementary polynucleotide strand).
Appropriate stringency conditions are known to those skilled in the art or may be determined experimentally by the skilled artisan. See, for example, Current Protocols in Molecular Biology, John Wiley & Sons, N.Y. (1989), 6.3.1-12.3.6; Sambrook et al., 1989, Molecular Cloning, A Laboratory Manual, Cold Spring Harbor Press, N.Y.; S. Agrawal (ed.) Methods in Molecular Biology, volume 20; Tijssen (1993) Laboratory Techniques in biochemistry and molecular biology-hybridization with nucleic acid probes, e.g., part 1 chapter 2“Overview of principles of hybridization and the strategy of nucleic acid probe assays”, Elsevier, New York; and Tibanyenda, N. et al., Eur. J. Biochem. 139:19 (1984) and Ebel, S. et al., Biochem. 31:12083 (1992).
The term “substantially homologous” when used in connection with a nucleic acid or amino acid sequences, refers to sequences which are substantially identical to or similar in sequence with each other, giving rise to a homology of conformation and thus to retention, to a useful degree, of one or more biological (including immunological) activities. The term is not intended to imply a common evolution of the sequences.
The term “patient” refers to a mammal in need of a particular treatment. In a preferred embodiment, a patient is a primate, canine, feline, or equine. In another preferred embodiment, a patient is a human.
Synthesis of Model Constructs of the 970 Hairpin Loop
The syntheses of the 6-O-DPC-2-N-methylguanosine (m2G) nucleoside and the corresponding phosphoramidite are reported. Among the two approaches used for the phosphoramidite synthesis, the 5′-O-DMT-2′-O-TOM-protected 6-O-DPC-2-N-methylguanosine phosphoramidite [DMT, 4,4′-dimethoxytrityl; TOM, [(triisopropylsilyl)-oxy]methyl; DPC, diphenyl carbamoyl] gave much higher yields. The availability of the phosphoramidite in sufficiently large quantities allowed for syntheses of hairpin RNAs with selective incorporation of 2-N-methylguanosine modification. Four 18-nt hairpin RNA analogues representing the 970-loop region (helix 31; U960-A975) of Escherichia coli 16S rRNA were synthesized with and without modifications in the loop region.
The 970 loop of helix 31 (h31) of E. coli 16S rRNA is located near the ribosomal P site and therefore believed to be intimately involved in translation.1-3. E. coli h31 contains two modified nucleotides, 2-N-methylguanosine at position 966 (m2G966) and 5-methylcytidine at position 967 (m5C967). The chemical synthesis of E. coli helix 31 therefore involves the incorporation of m2G and m5C modified phosphoramidites, in addition to the standard A, U, C, and G phosphoramidites. The m5C phosphoramidite is commercially available and was purchased along with standard (A, U, C, and G) phosphoramidites, while the m2G phosphoramidite was synthesized, which will be discussed in this chapter. Hence, chemical synthesis of the helix 31 RNA construct can be illustrated by a stepwise manner, which involves two major synthetic challenges as shown (
The first challenge was the synthesis of the methylated guanosine nucleoside, 2-N-methylguanosine (m2G). From the organic chemists' perspective, synthesizing m2G is challenging due to solubility problems encountered throughout the synthesis and purification steps. Commercially available m2G has a consistently high price. Currently, one milligram of m2G costs $40 at Sigma-Aldrich compared to $37 for 25 g of G. The commercially available m2G also requires further protection at the O6-position prior to phosphoramidite synthesis. In this work, the synthesis of m2G was achieved by using a combination of several published procedures. The next step was to synthesize the phosphoramidite of m2G in order to incorporate it into the oligonucleotide sequence of interest, namely helix 31. Two approaches were used to obtain the corresponding m2G phosphoramidite; one of which has given rise to higher yields in the m2G phosphoramidite synthesis than the methods reported previously. My first approach involved the synthesis of 5′-O-BzH-2′-O-ACE-6-O-DPC-2-N-methylguanosine phosphoramidite [BzH, benzhydryloxy-bis(trimethylsilyloxy)silyl; ACE, tris(2-acetoxyethoxy)orthoformate). Despite a successful small-scale synthesis, subsequent generation of this compound on a large scale was not achieved. In contrast, synthesis of the 5′-O-DMT-6-O-DPC-2-N-methyl-2′-O-TOM-guanosine-3′-(2-cyanoethyl)diisopropylphosphoramidite was accomplished on a large scale and therefore utilized in subsequent RNA syntheses. Since the m2G phosphoramidite of interest is not commercially available, its synthesis was quite useful for constructing the natural helix 31. The RNA hairpins used in this study were chemically synthesized at the W. M. Keck Foundation at Yale University, New Haven, Conn. USA. For RNAs containing m2G, 50 μmoles from the corresponding phosphoramidite were provided.
The synthetic protocol is described in further detail in the Examples. In summary, the synthesis of 2-N-methylguanosine (m2G) followed and adapted the methodologies from Matsuda and Reeses.4, 5 The lactam function (O6-position) of the guanine residue is protected according to a widely used procedure originally devised by Kamimura.8 In addition to the successful O6-protection of the guanine residue, introduction of DPC (diphenylcarbamoyl chloride) improves the solubility and chromatographic purification properties of the resultant derivatives. From this strategy, we were able to generate gram quantities of m2G from guanosine, which is relatively a cheap starting material.
Two approaches were used to obtain the corresponding m2G phosphoramidite, one of which gave high yields, allowing for gram quantities to be made. My first approach involved synthesis of the 5′-O-BzH-2′-O-ACE-6-O-DPC-2-N-methylguanosine phosphoramidite. Despite a successful small-scale synthesis, subsequent utilization of this compound in RNA synthesis was not achieved due to the inability to obtain the compound in sufficiently large amounts. Consequently, the synthesis of the 5′-O-DMT-6-O-DPC-2-N-methyl-2′-O-TOM-guanosine-3′-(2-cyanoethyDdiisopropylphosphoramidite was accomplished on a large scale and allowed us to generate RNAs for subsequent biophysical studies. Both MALDI-TOF mass spectrometric analyses and reverse-phase HPLC analyses of the enzyme digest products confirmed that the methyl group at the N2-position of guanosine remained intact during the chemical synthesis and deprotection strategies of helix 31 synthesis
Biophysical Characterization of the Helix 31 RNA Model Constructs
Biophysical investigations with model constructs representing helix 31 of E. coli and H. sapiens small subunit ribosomal RNA are discussed. Three types of biophysical techniques, namely circular dichroism, thermal melting, and nuclear magnetic resonance spectroscopy, were employed. The chemically synthesized E. coli RNA constructs were subjected to detailed biophysical analyses in order to reveal the possible roles of the modified nucleosides. Studies with an H. sapiens unmodified helix 31 RNA construct are also discussed. This work has led to the discovery of a novel and stable hairpin construct that can be used for future ligand-binding experiments.
Four constructs representing the helix 31 region of E. coli 16S rRNA, with and without modifications, were synthesized, as discussed above and in the examples. Our next goal was to reveal the ability of those constructs to represent helix 31 of 16S rRNA. Three different biophysical techniques were employed. UV melting experiments were performed to determine the stability of the stem regions; whereas, circular dichroism and 1D NMR spectroscopy were used to study structural features of the h31 RNAs. The imino proton peaks observed in 1D NMR spectra of the E. coli constructs were assigned using a 1D NOE difference spectroscopic analysis. The UV melting experiments also helped us to assign structural roles for the modified nucleosides present in this region.
The two methylated bases (m2G966 and m5C967) of E. coli helix 31 occur at the same or adjacent site as the hypermodified nucleotide 1-methyl-3-(3-amino-3-carboxypropyl)-pseudouridine (acp3m1Ψ) in the H. sapiens small subunit rRNA. Preliminary biophysical experiments were carried out with the unmodified version of human helix 31 in order to determine its ability to represent the natural hairpin structure. The stability of the original hairpin loop design was unusually low, generating reasonable doubt about its ability to represent the H. sapiens helix 31 region. This observation led us to perform a phylogenetic analysis to determine with other possible base pairs for the stem region of H. sapiens helix 31 RNA. The discovery of a novel construct to represent the H. sapiens helix 31 region and biophysical studies pertaining to this hairpin RNA will also be discussed in this chapter.
In summary, the significance of the E. coli modifications in h31 was explored by using various biophysical techniques. Modifications in the loop region of E. coli helix 31 are slightly destabilizing. Destabilization may allow helix 31 to be more flexible and to enhance its biological function.
The CD data indicate that the unmodified, singly modified, and fully modified RNAs all exist in solution as A-form helices and they display similar conformations. The presence of modifications at specific locations does not appear to influence the ability to form a hairpin structure. Furthermore, 1H NMR spectra of the h31 RNAs confirm the formation of three G-C base pairs and two A-U base pairs in the stem region; however, the presence of additional imino proton peaks in the NMR spectra with differing chemical shifts for each h31 model RNA suggests the formation of alternate loop conformations or dimerization artifacts. The residual peaks (marked by * in
Overall, there is good agreement between the ID NMR data and the thermal melting data. Loss of the imino peak corresponding to the g1-c18 base pair of ECh31WT is consistent with a lowering of the Tm and hence the decreased stability of the RNA construct.
The exact functional role of the modifications at positions 966 and 967 of h31 is still unknown. Ribosomes carry out the essential biochemical process of translation, which requires an exquisite array of highly specific interactions between rRNA, mRNA, tRNAs, and ribosomal proteins. Modifications are believed to help fine-tune ribosome function.18 Since proper ribosome function depends on the correct balance of speed and accuracy of tRNA binding, peptide-bond formation and tRNA release, methylations in h31 could play a role in maintaining proper interactions within the ribosome.19, 20 Mutational analyses revealed that a loss of methylation at either position 966 or 967, leads to increased protein production by the mutant ribosomes.21 Our data would therefore suggest that methylations destabilize h31 in order to maintain the proper interactions with tRNA, rRNA, or proteins. A lack of modification at residues 966 or 967 in h31 could reduce the ability of base 966 to flip and regulate tRNA affinity, positioning, or accuracy.
Reconstruction of the human analogues of helix 31 with the E. coli stem made it more stable for biophysical studies and hence proved to be suitable for the future ligand binding studies. According to CD studies, differences in both peak maxima and peak minima for HSh31ECstem and ECh31UNMOD are significant even though they both have the same stem sequences. This result implies that the loop regions are influencing the structures of these two analogues. UV melting data suggest that the loop region corresponding to the H. sapiens rRNA h31 exerts a destabilizing effect on the stem relative to the E. coli loop region, irrespective of the fact that they have the same number of nucleotides (eight) in their loop regions and both share the same base-pairing schemes in the stem region. These data are consistent with the CD results.
Identification of Peptides Targeting Helix 31
The ribosome is a protein-synthesis machine that has been used as a drug target for decades. Ribosomal RNA is the catalytic part of the ribosome. It can undergo different conformational changes during translation, which can be facilitated by modified nucleotides. A phage-display experiment was carried out to select for peptides that bind to helix 31 of the 16S ribosomal RNA of Escherichia coli. Helix 31 harbors two modified nucleotides, m2G966 and m5C967, which are conserved in each of the phylogenetic domains. The degree and nature of modification is different in prokaryotes and eukaryotes. By using modified and unmodified variants of h31 as targets in a phage-display experiment, consensus peptide sequences were isolated after several rounds of screening. Their inhibitory effects on protein synthesis were identified by using in vitro protein translation assays.
Intermolecular interactions are important in all cellular processes, such as transcription, translation, and cell signaling. Protein-protein, protein-DNA and protein-RNA interactions are crucial events in the cell. As soon as the RNA is transcribed, ribonucleoproteins (RNPs) bind to the nascent transcript and carry out RNA processing, nuclear export, transport and localization (5). Understanding the basic principles of RNA-protein interactions is important for the identification of ligands that recognize specific structures, or motifs of RNA.
RNA-protein interactions. RNA-protein interactions are a fundamental process of gene regulation in every living organism (8). Such types of interactions are facilitated by RNA's ability to form diverse secondary structures such as bulges, hairpins, pseudoknots, and A-form helices. The ribosome contains many examples of RNA-protein interactions in which the functional conformations of ribosomal RNA (rRNA) are achieved only after interactions with ribosomal proteins. In many cases, although RNA recognition is mediated by highly basic stretches of amino acids that are rich in arginine and lysine residues, the presence of these residues is not usually sufficient to recognize specific RNA motifs (9, 10). Among the 11 different types of RNA-binding domains present in nature, the single-stranded RNA-binding domain (ssRBD) and double-stranded RNA-binding domain (dsRBD) are the most abundant (11). The RNA-recognition motif (RRM), the K homology domain (KH), and the oligonucleotide/oligosaccharide binding-fold domain (OB-fold) are common examples of ssRBDs. RRM is a well-characterized domain. More than 6000 RRM sequences have been discovered, and almost 2% of the human genome has RRM motifs (12). Double-stranded RNA-binding proteins contain 70-90 amino-acidlong, RNA-binding-motifs and are found in both bacteria and eukaryotes. The dsRBD binds across two successive minor grooves and an intervening major groove on one face of double-stranded RNA helices (13) (
Identification of molecules targeting RNA. Regions in the RNA where there are perturbations in the A-form helices are optimal sites for RNA targeting. The standard major and minor grooves of RNA are not optimal binding sites for small molecules. Once an ideal targeting site is identified, the next goal is to determine the class of compounds to consider for potential ligands. Clinical trials of many small molecules have been unsuccessful due to their toxicity, even if they have low costs, long half lives, and are easy to synthesize (18). With the development of new technologies, peptide-based drugs are taking the leading role in drug discovery and are now viable alternatives to antibodies and small molecules as potential drugs. Peptides have some advantages over small molecules such as ease of tissue penetration, high specificity, and low toxicity (19).
Some drawbacks such as short half life, susceptibility to protease degradation, low permeability through cell membranes, and low transport through the blood-brain barrier limit their usefulness as drug candidates (19). By using peptidomimetic chemistry, the functional groups and backbones of the peptides can be changed to overcome these problems. Highly structured peptides including cyclic, α helical, and β sheet-like motifs usually have higher affinities for their targets. Usually, heterodimer peptides have better abilities to block protein-protein or protein-RNA interactions because they occupy larger surface areas, enough to disrupt the bridges between two molecular surfaces (20). These dimer peptides could be better therapeutic agents than small molecules and antibodies because of such desirable properties (21).
High-throughput screening (HTS) methodologies have been used to identify peptides from synthetic or biological libraries (22). Today, more than 140 peptides have been used as drugs and more than 400 peptides are in various phases of clinical trials (Table 1) (1). The number of peptides being used as drugs increases by approximately 15% per year (1). Without prior knowledge of their structures, the peptides can be screened for better affinity to the target (23). Different biological peptide libraries can be constructed by using molecular genetics and recombinant display technologies, such as ribosome display (24), phage display (25), mRNA display (26), and cell display (27). These techniques enable the identification of high affinity peptides with a K.sub.ds<10 nM against different targets (21, 28).
Phage display. Since discovery of the phage-display technology by George Smith in 1985 (25), it has been used extensively in the pharmaceutical industry for drug discovery. It has been used to isolate ligands for drug discovery (29), affinity chromatography (30, 31),
TABLE 1
Examples of therapeutic peptides used in clinical trials are
listed. This table is adapted from Huther A et al; 2007.
Peptide drugs
Company
Peptide length
Therapy
Clinical status
Enfuvirtide
Trimeris/Roche
36
Anti-HIV
Approved
Fusion inhibitor
Hematide
Affymax
20
Erythropoietin mimetic
Phase II
Anemia
Dentonin
Acologix Inc.
23
Stimulation of dental pulp stem
Phase II
cell proliferation
Insulin
Eli Lilly
51
Type I diabetes
Approved
Byetta
Amylin/Eli Lilly
39
Type II diabetes
Approved
Ostabolin C
Zelos Therapeutics
31
Osteoporosis
Phase II
DiaPep277
DeveloGen AG
24
Type II diabetes
Phase II
Exubera
Pfizer
???
Type I & II diabetes
Phase II
(Non-injectable insulin)
epitope mapping of antibodies (32, 33), protein-protein interactions (34-36), isolating antibody fragments (35, 36), engineering the binding affinity of displayed proteins (37, 38), identification of peptides that target organs or tissues (39, 40), enzyme inhibition (29), as well as many other applications. The basis of this technology is the construction of a library of various peptides fused to one of the coat proteins of bacteriophage. The DNA encoding the peptide resides inside the bacteriophage genome providing a linkage between a phenotype and genotype, in which peptide sequences can be easily identified by sequencing the phage DNA (41). Highly diverse phage-displayed peptide libraries (approximately 109) are commercially available. A library with randomization of codons of seven amino acids contains approximately 3.4×1010 unique sequences (327, NNK=41×41×21, where K=C, T), which represents 1.39×109 (207) unique amino acid combinations. Even a library with 1010 unique members is unlikely to provide complete coverage of all possible sequences.
M13 and T7 bacteriophage are commonly used in phage display. M13 is a non-lytic, filamentous bacteriophage (42). Since it does not lyse the bacterial cells, there is minimal chance of contamination due to bacterial proteases and nucleases during the course of selection. Other advantages of M13 are its stability and resistance to high temperature (55° C.) and acidic conditions (pH 3.0) (43). M13 phage is composed of circular ssDNA (6407 nucleotides) that is encapsulated by different major and minor coat proteins (
The typical procedure for affinity selection includes immobilization of target molecule on the surface of beads or in the wells of microtiter plates (
The eluted phage are infected into specific bacterium to amplify the sub-population of phage before going to the next cycle of selection. After three to five cycles of selection, target-specific and tightly bound peptides are isolated (2).
Identification of peptide ligands using RNA as a drug target. After the discovery of phage display in 1985, most of the work that followed involved the isolation of ligands using protein as the target. The use of phage display to target RNA picked up momentum nearly one decade after its discovery (47, 48). Peptides isolated from the library can mimic the specific motifs of proteins, which are important for recognization of RNAs such as Tar and RRE from HIV (49, 50). Under physiological conditions, the shorter peptides may lack any secondary structure; however, they may still have specific interactions with RNA (51). X-ray crystallography and NMR structures of peptide-RNA complexes have provided further insights into peptide-RNA interactions (52). U1 RNA-binding antibody fragments were isolated from autoimmune human-derived bacteriophage display libraries (53, 54). Peptide ligands for psi RNA from the HIV-1 packaging signal were identified and their specificity was characterized (55, 56). Agris' lab isolated modified-nucleotide-specific peptides by using the anticodon stem-loop region of different tRNAs as the targets (57-60). To date, no work has been published on targeting the modified nucleotides of ribosomal RNA.
Modified rRNA as a drug target. It has been shown that the absence of certain modifications in tRNA abolishes the recognition of tRNA-synthetase as well as initiation and elongation factors. The presence of modified nucleotide 1-methylguanosine at residue 37 (m1G37) in tRNAAsp and lysidine in the anticodon of E. coli tRNAIle prevents mis-aminoacylation of near-cognate amino acid (61, 62). In some cases, loss of modifications in bacterial ribosomal RNA leads to resistance or sensitivity to antibiotics, indicating that ligand-RNA interactions are mediated either directly or indirectly by modified nucleotides (63, 64). These facts highlight the possibility of using modified RNA as a potential drug target.
Helix 31 (970 loop) of the bacterial 16S ribosomal RNA, which contains two modified nucleotides, m2G966 and m5C967 (
Using both modified and unmodified h31 as targets (
In summary, RNA-protein interactions are very crucial for biological processes. RNA function is regulated by RNA-binding proteins, which also control gene expression. A peptide that can disrupt critical interactions by binding to a specific RNA motif inside the cell can be a potential drug lead. Several RNA-binding peptides have been discovered by phage display, and it was found that they recognize and bind to specific motifs of RNA structure (10). RNA modifications play a significant role in efficient protein-RNA interactions (80). Several studies (including this thesis work, Chapters 2, 3 and 4) have shown the importance of modifications in different aspects of protein synthesis, such as translational fidelity, ribosome assembly, stability and initiation.
One of the current challenges in medicine is the rapid development of drug resistance due to target-site mutations. Therefore, if we can identify new drugs that target essential modified nucleotides or RNA regions, this problem might be solved in the future. By using phage display, peptide motifs recognizing the RNA with modified nucleotides can be identified and they can be used as drug leads.
Helix 31 plays an important role in protein synthesis (81, 82). From several biochemical and structural studies, it has been shown that modified nucleotides m2G966 and m5C967 are close to the P-site tRNA and mRNA (83, 84). This helix also interacts with S9 and S10 ribosomal proteins and initiation factor 3 (1F3) (67, 81, 85). The loss of modifications affects translational fidelity and interactions with initiation factors. One more significant feature of this loop is the domain-specific phylogenetic conservation of modifications (65, 66), suggesting its importance as a potential drug target. If we can identify ligands (peptides) that can interrupt the essential interactions of h31 and tRNA, mRNA, or initiation factors by specific recognition of this bacterial rRNA loop, those molecules could potentially be used as drug leads.
Synthesis and Characterization of Peptides that Target Helix 31
Solid-phase syntheses of peptides that were selected against helix 31 in the bacterial ribosome are discussed. Availability of the chemically synthesized peptides allowed us to characterize their affinities with helix 31 using various biophysical techniques. Biophysical characterizations by circular dichroism, fluorescence spectroscopy, and surface plasmon resonance are discussed. This work revealed two high-affinity peptides that have nanomolar affinities toward bacterial helix 31 RNA.
The chemical syntheses of bacterial h31 model constructs allowed us to reveal not only the possible roles of the modifications present in this region, but also allowed us to subject this construct to phage-display screening experiments (performed by Tek Lamichhane in collaboration with the Cunningham lab). Phage display is a selection method that allows for the identification of peptides from a random library of sequences that have affinity for a chosen target.1-3 Consequently, several peptide sequences were obtained with potential for recognition of the h31 region in the bacterial ribosome. In order to further investigate the peptide affinities and specificity towards h31, it was necessary to obtain those peptides via a chemical synthetic strategy. Two major methods are reported in the literature for the chemical synthesis of peptides, namely solution-phase and solid-phase peptide synthesis.4 Among the two methods, solid-phase peptide synthesis (SPPS) has become the most useful methodology due to its simplicity. SPPS was first established by Robert Bruce Merrifield in 1963,5 and he was awarded the Nobel prize for his outstanding work in 1984.4
SPPS has become our choice for obtaining the phage-display selected peptides, not only due to its simplicity, but also due to its compatibility with our system and the ability to obtain large amounts of peptide with few by-products. In order to achieve successful SPPS, it is desirable to choose an adequate combination of protecting groups/solid support before commencing a synthesis. For routine syntheses, the choice is generally limited to Fmoc/tBu-6-7 or Boc/benzyl5, 8-based methodologies [Fmoc, 9-fluorenylmethoxycarbonyl chloride (Fmoc-Cl); Boc, di-tert-butyl pyrocarbonate]. The chemical structures of Fmoc and Boc protecting groups are given in
During our syntheses, we used the Fmoc/tBu-type chemistry. The Fmoc/tBu-based SPPS process is summarized in
During our experiments, the peptides were obtained by SPPS using a manual synthetic apparatus in which the reactor consists of a cylindrical vessel with a fritted disk and a screw cap lid (
A typical vessel used in our synthesis is six inches in height and has an internal diameter of one inch. These are custom-made glass vessels and proper care must be used during handling. The upper-end can be capped with a Teflon screw-cap lid; whereas, the solvent flow through the bottom is controlled by a stop-cock. Just above the stop-cock, there is a fritted-disk that retains the resin. When the stop-cock is in the closed position, the vessel can retain both the resin and the solvent containing other reagents. A constant shaking is applied by a mechanical stirrer. This step allows the coupling reaction to take place. But when the stop-cock is open and the bottom end is connected to a vacuum generator, the solvent and reagents are filtered through while leaving the resin on the surface of the fritted disk. This step allows a new round of amino-acid coupling to be performed on the resin with a new set of reagents. In order to perform an effective synthesis, an appropriately functionalized resin (polymer support) is chosen. The resin is made out of polystyrene, and is often functionalized with linkers that serve as actual coupling ends.9 The choice of the linker, and hence the resin, depends on the conditions necessary for the synthesis, the cross reactivity with different reactant functionalities, and special requirements for the particular synthetic route, etc. The most common functionalities on the linkers are alcohols, aldehydes, acids, amines, thiols, and chlorines.9
During the phage-display screening process, the C-termini of the peptides are not free. On M13 phage, the peptides are displayed with free N-termini exposed to the environment. The C-termini are linked to the minor coat protein (P3) of M13 phage through a short spacer forming an amide bond. In order to mimic this type of display, the peptides were chemically synthesized on Rink Amide resin (
The Rink amide resin was obtained in its Fmoc-protected form for our syntheses. Therefore, the first step of the synthesis involved removal of the Fmoc protecting group under mild basic conditions with 25% piperidine in DMF.9 A similar strategy was used to remove Fmoc protections from all amino acids immediately after their coupling step (
Fmoc deprotection exposes the free amino terminus for subsequent coupling with the incoming Fmoc-protected amino acid. Coupling reactions were performed with a 0.05 M solution of the Fmoc-protected amino acid, 1-hydroxy-1H-benzotriazole (HOBt),10 and N,N′-diisopropylcarbodiimide (DIC)11 in DMF. The addition of DIC activates the carboxylic group of the incoming amino acid, while HOBt is used as the catalyst. In the absence of HOBt, the situation is totally different. Racemization can occur due to high reactivity of the carboxylic acid activator, DIC.10 This causes cyclization of the activated species to an oxazolone, which racemizes via enolization and subsequent reopening by the amino component to yield epimers (
For this reason, a second reagent (HOBt) is added which displaces DIC upon activation of the incoming amino acid (FIG. 76).10 HOBt acts as an auxiliary nucleophile. It forms an O-acyl-1-hydroxy-benzotriazone upon transesterification of the highly active amino-acyl-isourea species formed by the reaction between the amino acid and DIC. This step suppresses the racemization by shortening the lifetime of the amino-acyl-isourea species.10 A detailed mechanism for the HOBt/DIC mediated amino acid coupling is given in
The progress of the coupling reactions and deblocking steps are monitored by the Kaiser test (FIG. 77).13, 14 It is based on the reaction between ninhydrin and amine groups. This is a qualitative test for the detection of primary amines, visualized by an intense blue color (Ruhemann's blue), and therefore may not provide reliable information in the presence of secondary amines such as proline and other N-substituted amino acids. Those may generate a brownish red color from the test.
The Kaiser test provides a negative result only when the coupling reaction has gone to completion. Otherwise, it shows an intense blue color indicating that the reaction is in an intermediate stage. This particular feature of the Kaiser test is rather useful in peptide synthesis, as it is indicative of the 100% efficiency in each coupling step.
The coupling step is repeated until the desired peptide sequence is obtained. Then, peptide cleavage from the resin and deprotection of the amino-acid side chains are achieved with a mixture of trifluoroacetic acid (TFA)/triisopropylsilane (TIS)/anisole/thioanisole (94:2:2:2, vol:vol:vol:vol).15, 16 During the final cleavage step, highly reactive carbocations are generated; it is therefore necessary to trap them in order to avoid side reactions with sensitive amino acids such as Cys, Met, Ser, Thr, Trp, and Tyr.15 This step is achieved by the addition of scavengers such as water, anisole, thioanisole, TIS, etc. At the final step, the resin is filtered off and the solution containing the crude product is drained into cold diethylether (Et2O). The resulting cloudy mixture is centrifuged and lyophilized. The crude peptides are purified by semi-preparative HPLC. Characterization of the peptides is done by MALDI-TOF mass spectrometry.
Several conclusions can be drawn from the work reported in this chapter. Among the methods utilized for the peptide-RNA binding characterization, CD and fluorescence have provided good starting points for the future peptide binding experiments. Despite the poor curve fit obtained for the fluorescence titration experiment, the data gave us some hope for the subsequent experiments. Several reasons can be put forward for the low reliability of the fluorescence data. Problems associated with the RNA construct (fluorescein is attached to the guanosine residue at 5′ end of the RNA) might have caused the fluorescence intensity to be quenched, hence resulting in a small percentage of reduction in the fluorescence intensity. On the other hand, peptide aggregation effects at higher concentrations might have resulted in poor curve fitting. Data analyses assuming a coorporative binding mode generated inferior fits than the one that is reported.
Circular dichroism data has provided a comparable value for the dissociation constant with a greater margin of error. That may possibly be due to the discrepancies in the isodichroic point, which is indicative of peptide aggregation effects. Despite a greater margin of error, both of the above-mentioned techniques provided a comparable dissociation constant for the interaction of 17 (TYLPWPA (SEQ ID NO: 2)) with h31 RNA.
When the same system, 17 (TYLPWPA (SEQ ID NO: 2)) with h31 RNA, was further analyzed to reveal the kinetics of the interaction, the dissociation constant was comparable to that obtained from CD and fluorescence. In the SPR analysis, the peptide was cloned with GFP to gain a better signal-to-noise ratio. Despite the presence of GFP, the dissociation constant of 17 (TYLPWPA (SEQ ID NO: 2)) with h31 RNA was found to be consistent with the values obtained from other two techniques. The SPR analysis provided a dissociation constant with a lower margin of error. Therefore, SPR has provided a better platform for the studies of peptide-RNA interactions with greater reliability. One intriguing question is the affinity of GFP itself towards h31 RNA. This affinity might presumably be required in this kinetic investigation to bring the peptide towards the RNA. This situation would be comparable to that one might observe in the phage-display technique, in which the peptide is associated with the phage during the selection process. Therefore, we can argue that a similar scenario has been created for the peptide when it is attached to GFP. The GFP may not only bring the peptide close to its target, but it may also be limiting the conformational flexibility of the peptide in a favorable manner for the observed binding. The utility of SPR technology in the peptide-RNA binding studies was further revealed by studies with peptides 14 (TLWDLIP (SEQ ID NO: 3)) and 15 (CVRPFAL (SEQ ID NO: 4)) with h31 RNA. The two peptide conjugates have nanomolar affinities for h31. This result was further validated by a coupled in vitro transcription-translation assay performed by Tek Lamichhane (in collaboration with the Cunningham lab). Based on the results of this experiment, the two nanomolar affinity peptides (14 and 15) have shown greater inhibitory effects on in vitro protein synthesis than other peptides that were obtained from the phage-display selection (
A peptide ligand/s that can bind specifically to the h31 region of E. coli 16S rRNA was discovered. Therefore this region may be utilized as a potential drug target in the bacterial ribosome. The availability of the wild-type h31 RNA construct allowed us to discover peptide sequences that possess high affinity and specificity towards this region, may lead to the discovery of yet another anti-infective target in the bacterial ribosome.
Peptides of the Invention
In certain embodiments, the invention relates to peptides discussed in the Examples.
In certain embodiments, the invention relates to a peptide with the sequence: TLWDLIP (SEQ ID NO: 3).
In certain embodiments, the invention relates to a peptide with the sequence: CVRPFAL (SEQ ID NO: 4).
In certain embodiments, the invention relates to a peptide with the sequence: ATPLWLK (SEQ ID NO: 5).
In certain embodiments, the invention relates to a peptide with the sequence: TYLPWPA (SEQ ID NO: 2).
In certain embodiments, the invention relates to any one of the aforementioned peptides, wherein the conventional single letter abbreviations are used.
In certain embodiments, the inventino relates to the D-, Beta, or peptoid verions of any one of the aforementioned peptides.
Structural Studies of Targets and Compounds
Interactions of the hits (peptides and compounds) and drug leads with their E. coli rRNA targets are characterized using NMR spectroscopy to determine key functional groups important in the interaction. This data is helpful in modifying the drug leads using rational drug design and medicinal chemistry to improve bioavailability, pharmacodynamics, and to reduce toxicity.
NMR studies provide several types of critical information. First, NMR is used to verify whether the structure of isolated RNA targets taken out of the context of the ribosome resemble their structure in the ribosome and will therefore be valid targets for screening compound libraries. NMR spectroscopy also provides detailed stereochemical information on the mechanism of binding of small-molecule ligands with RNA targets. Lastly, NMR studies reveal crucial differences between the E. coli and the human small subunit rRNAs. Comparison of the wild-type and mutant structures will reveal the essential functional groups and structural folds required for ribosome function, thereby focusing the design of drugs to these critical residues. Structural characterization of RNA-ligand complexes will reveal how each compound recognizes the essential target motifs. Further, characterization of RNA dynamics by NMR in the presence and absence of bound drug leads will reveal the role of induced fit in RNA recognition. [Chow, C. S. & Bogdan, F. M. (1997). A Structural Basis for RNA-Ligand Interactions. Chem. Rev. 97, 1489-1513.]
Target Validation
Potential drug compounds are tested in eukaryotic and bacterial in vitro protein synthesis assays. Compounds that inhibit wild-type and mutant bacterial ribosomes but not eukaryotic ribosomes are further developed, and allow in vitro validation of the selected targets.
In another embodiment, the functionally important regions identified above are divided into groups based upon whether or not they occur in closely related groups of organisms. For instance, some regions of rRNA are found in all bacteria but not in other organisms. Other areas of rRNA are found only in closely related groups of bacteria, such as all of the members of a particular species, e.g., members of the genus Mycobacterium or Streptococcus.
In a further embodiment, the regions found in very large groups of organisms, e.g., all bacteria or all fungi, are used to develop broad-spectrum antibiotics that may be used to treat infections from a large number of organisms within that group. The methods of the present invention may be performed on these regions and functional mutant ribosomes identified. These functional mutant ribosomes may be screened, for example, with compound libraries.
In yet another embodiment, regions that are located only in relatively small groups of organisms, such as all members of the genus Streptococcus or all members of the genus Mycobacterium, may be used to design narrow spectrum antibiotics that will only inhibit the growth of organisms that fall within these smaller groups. The methods of the present invention may be performed on these regions and functional mutant ribosomes identified. These functional mutant ribosomes will be screened with, e.g., compound libraries.
Methods of the Invention
One aspect of the present invention relates to a peptide obtained as described herein. Yet another aspect of the present invention relates to a method of administering to a patient in need thereof a peptide and/or compound obtained by any one of the aforementioned methods, wherein said patient is suffering conditions associate with a microbial infection, such as an infection caused by, for example, E. coli, P. aeruginosa, or the like. In certain embodiments said microbial infections is a bacterial infection.
The invention now being generally described, it will be more readily understood by reference to the following examples, which are included merely for purposes of illustration of certain aspects and embodiments of the present invention, and are not intended to limit the invention.
General Procedures for Examples 2-5
Most reagents and solvents were either purchased from Aldrich (St. Louis, Mo.) or Across (Morris Plains, N.J.). Benzhydryloxy-bis(trimethylsiloxy)silyl chloride (BzHCl), 4-(tert-butyldimethylsilyloxy)-3-penten-2-one (TBDMS-pent), and tris(2-acetoxyethoxy)-orthoformate (ACE) were purchased from Dharmacon, Inc. (Lafayette, Colo.). All other reagents and solvents were purchased form commercial sources and used as received. Anhydrous pyridine was purchased in a sure-seal bottle from Aldrich. Methylene chloride (CH2Cl2) was distilled over CaH2. Methanol and triethylamine was purchased dry from Aldrich in a sure-seal bottle. Moisture sensitive reactions involved flame-drying equipment (syringes, round-bottom flasks, stir-bars, etc.) under vacuum and performing reactions under dry argon. TLC analyses were accomplished with precoated silica gel (0.25 mm thickness) glass plates. Reactions were monitored by visualizing the TLC plates under UV light and/or by staining with phosphomolybdic acid (PMA) solution (10% w/v in absolute ethanol). Flash chromatography was performed with silica gel 60 (0.038-0.063 mm). Flash columns were neutralized with 0.5-1% triethylamine (TEA) prior to purification of pH sensitive intermediates/compounds. 1H NMR and 13C NMR spectra were recorded on either a Varian Unity 300, Mercury 400, or Varian Unity 500 spectrometer and referenced to tetramethylsilane as an internal standard. ESI spectra were recorded on a Quattro LC (Bruker Daltonics) in the positive ion mode unless otherwise noted.
NMR methods. Sample (20-40 mg) was dissolved in the deuterated NMR solvent (˜3 mL) to obtain a clear solution. The samples were either sonicated or filtered through a cotton plug, when ever insoluble particles were observed. CDCl3 was neutralized by passing through basic alumina to avoid any degradation of acid-sensitive compounds.
MALDI-TOF mass spectrometric methods. The sizes of the chemically synthesized RNAs and the presence of the methyl modifications were confirmed using MALDI-TOF mass spectrometry. The samples were prepared by mixing 5 μl supersaturated matrix solution (3-hydroxypicolinic acid in dH2O/acetonitrile, 50/50 V/V), 0.5 μl RNA (5-10 pmol), and 0.5 μl 100 mM NH4OAc. Next, 1 μl of the mixture was spotted on a MALDI plate and dried in the air. The RNA samples were then analyzed on a Bruker Ultraflex MALDI-TOF under negative ion mode and linear acquisition operation mode.
HPLC methods. Confirmation of nucleosides present in the synthetic RNAs were obtained by digestion of ˜0.5 ODs of RNAs to their corresponding nucleotides with P1 nuclease [1.5 units], 0.5 M NaOAc [Cf=37.5 mM], 5 mM ZnCl2 [Cf=0.25 mM], at 37° C. overnight. The mixtures were then heated at 70° C. for 15 min (to inactivate P1). Then, the samples were cooled on ice. The corresponding nucleosides were then obtained by treating the resulting nucleotides with CIP (calf intestinal phosphatase) [1.5 units], 0.5 M Tris.HCl, pH 8.3 [Cf=56 mM], at 37° C. for 2 h. Then, the mixtures were heated to inactivate CIP, and the resulting mixtures were filtered through microcon (Millipore, MWCO 30,000) and analyzed by reverse-phase HPLC on a Supelco C18 column. Approximately 0.25 OD were injected for each analysis. A linear gradient in 0.1 M TEAA buffer, pH 6.0 from 0 to 30% methanol over 17 min at a flow rate of 1 mL/min was employed. The retention times of the nucleosides were confirmed by injection of authentic standards (C=6.7 min, U=9.6 min, m5C=12.7, G=16.1 min, m2G=19.4 min, A=19.9 min).
The RNAs were purified by HPLC on an XTerra MS C18 column (2.5 μm, 10×50 mm, Waters) in which the eluent was 0.1 M TEAA buffer, pH 7.0, with a 5-15% linear gradient of acetonitrile over 25 min. at a flow rate of 4.0 mL/min. The column was pre-equilibrated with 80% of buffer A (5% acetonitrile in TEAA) and 20% of buffer B (15% acetonitrile in TEAA) prior to sample introduction. The elution of RNA was monitored by a photodiode array (PDA) detector scanning at a wavelength of 254 nm.
In general, the methylated guanosine nucleoside, m2G, was synthesized by using a combination of several published procedures (
Specifically, the synthesis was carried out as follows:
2′,3′,5′-Tri-O-acetylguanosine [1]. To a colloidal suspension of guanosine nucleoside (105 mg, 0.37 mmol, 1.0 eq) and 4-dimethylaminopyridine (4 mg, 0.03 mmol, 0.08 eq) in acetonitrile (5 mL) and triethylamine (0.2 mL, 1.51 mmol, 4 eq) was added the acetic anhydride (0.12 mL, 1.3 mmol, 3.6 eq) at room temperature. The suspension was stirred for 30 min. Then methanol (5 mL) was added to the mixture and stirring was continued for another 5 min. The mixture was evaporated to dryness under reduced pressure. The residue was chromatographed on a column of silica gel to give 1 as an off-white solid in 99% yield (152 mg, 0.37 mmol). TLC (CH2Cl2:MeOH, 9:1 v/v): Rf=0.37; 1H NMR (DMSO-d6, 400 MHz) δ (ppm): 2.01 (s, 3H), 2.02 (s, 3H), 2.08 (s, 3H), 4.22-4.28 (m, 1H), 4.33-4.37 (m, 1H), 5.48 (dd, J=4, 6 Hz, 1H), 5.76 (t, 1H), 5.95 (d, J=6 Hz, 1H), 6.5 (br.s, 1H), 7.85 (s, 1H), 8.2 (s, 1H), 10.7 (br.s, 1H); 13C NMR (DMSO-d6, 400 MHz) δ (ppm): 20.1, 20.3, 20.4, 62.95, 70.25, 72.04, 84.46, 116.85, 135.41, 150.97, 153.79, 156.65, 168.96, 169.13, 169.79; ESI-MS (ES+) calculated for C16H19N5O8 409.1234, found 410.2 (M+H+), 432.1 (M+Na+), 448.1 (M+K+), 841.3 (2M+Na+).
2′,3′,5′-Tri-O-acetyl-2-N-(p-methylphenylthiomethyl)guanosine [2]. 2′,3′,5′-Tri-O-acetylguanosine 1 (4.6 g, 11.2 mmol, 1.0 eq), 37% aqueous formaldehyde (4.7 mL, 156 mmol, 14 eq), p-thiocresol (4.6 g, 37 mmol, 3.3 eq), and acetic acid (2 mL) were added into 50 mL of ethanol. The mixture was heated under reflux for 4 h. The mixture was cooled and the white precipitate was collected by filtration. Product was recrystallized from water to obtain the pure solid compound 2 in 75% yield (4.58 g, 8.4 mmol). TLC (CH2Cl2:MeOH, 9:1 v/v): Rf=0.57; 1H NMR (DMSO-d6, 400 MHz) δ (ppm): 2.03 (s, 6H), 2.09 (s, 3H), 2.25 (s, 3H), 4.26-4.29 (m, 1H), 4.30-4.34 (m, 1H), 4.9 (br.s, 2H), 5.48 (br.s, 1H), 5.77 (t, 1H), 5.97 (d, J=6.4 Hz, 1H), 6.1 (br.s, 1H), 6.54 (br.s, 1H), 7.11 (d, J=7.2 Hz, 2H), 7.3 (d, J=7 Hz, 2H), 7.9 (s, 1H), 10.7 (br.s, 1H); 13C NMR (DMSO-d6, 400 MHz) δ (ppm): 20.2, 20.4, 20.5, 63.5, 67.2, 70.3, 72.06, 79.55, 84.44, 129.53, 129.54, 135.67, 153.94, 156.69, 169.31, 169.49.
2′,3′,5′-Tri-O-acetyl-2-N-methylguanosine [3]. Sodium borohydride (625 mg, 16.5 mmol, 1.82 eq) was added to a solution of 2′,3′,5′-tri-O-acetyl-2-N-(p-methylphenylthiomethyl)guanosine 2 (5.0 g, 9.2 mmol, 1.0 eq) in dimethyl sulfoxide (25 mL). The mixture was heated at 100° C. for 1 h and then cooled to room temperature. Reaction products were neutralized with 1 M aqueous potassium dihydrogen phosphate solution. The precipitate obtained was collected by filtration and further washed with acetone. The residue was chromatographed on a column of silica gel to give 3 in 75% yield (2.93 g, 6.93 mmol). TLC (CH2Cl2:MeOH, 9:1 v/v): Rf=0.45; 1H NMR (DMSO-d6, 400 MHz) δ (ppm): 1.92 (s, 3H), 2.03 (s, 3H), 2.04 (s, 3H), 2.8 (d, J=4 Hz, 3H), 4.11-4.15 (dd, J=6, 11.6 Hz, 1H), 4.23-4.25 (m, 1H), 4.33-4.37 (dd, J=4, 11.6 Hz, 1H), 5.7 (t, 1H), 5.8 (t, 1H), 5.9 (d, J=4 Hz, 1H), 6.4 (q, 1H), 7.79 (s, 1H), 10.79 (s, 1H); 13C NMR (DMSO-d6, 400 MHz) δ (ppm): 20.2, 20.3, 27.7, 40.4, 62.7, 69.7, 72.1, 78.5, 86.4, 117.3, 136.9, 150.2, 153.3, 156.6, 169.3, 169.4, 169.9; ESI-MS (ES+) calculated for C17H21N5O8 423.139, found 424.2 (M+H+), 446.2 (M+Na+), 847.3 (M+H+), 869.3 (2M+Na+).
2-N-Methyl-6-O-(diphenylcarbamoyl)guanosine [5]. To a solution of 2′,3′,5′-tri-O-acetyl-2-N-methylguanosine 3 (3.0 g, 7.1 mmol, 1.0 eq) in dry pyridine (50 mL) were added diphenylcarbamoyl chloride (3.45 g, 15 mmol, 2.1 eq) and diisopropylethylamine (1.9 mL, 11.4 mmol, 1.6 eq). The dark brown reaction mixture was then stirred at room temperature for 1 h to obtain 2′,3′,5′-tri-O-acetyl-6-O-(diphenylcarbamoyl)-2-N-methylguanosine 4. TLC showed complete conversion at this stage of the reaction. The reaction mixture was then diluted with pyridine (15 mL) and EtOH (30 mL). To this solution cooled at 0° C. was added 2 M NaOH (25 mL), which was precooled at 0° C. The reaction mixture was stirred for 10 min at 0° C. Acetic acid (c.a. 5 mL) was then added to neutralize the solution. Extraction with CH2Cl2 followed by chromatography on silica gel afforded 5 in 55% yield (1.92 g). TLC (CH2Cl2:MeOH, 9:1 v/v): Rf=0.5; 1H NMR (DMSO-d6, 400 MHz) δ (ppm): 2.81 (d, 3H), 3.51-3.56 (m, 1H), 3.61-3.66 (m, 1H), 3.90 (m, 1H), 4.02 (q, 1H), 4.15 (br.d, 1H), 4.62 (br.s, 1H), 4.99 (br.s, 1H), 5.21 (d, J=4.8 Hz, 1H), 5.48 (d, J=5.6 Hz, 1H), 5.82 (d, J=5.6 Hz, 1H), 7.28-7.32 (m, 4H), 7.4-7.44 (m, 6H), 8.19 (s, 1H); 13C NMR (DMSO-d6, 400 MHz) δ (ppm): 28.3, 61.5, 70.5, 73.1, 85.5, 116.4, 127.1, 129.4, 140.9, 141.8, 150.4, 155.6, 155.9, 159.6; ESI-MS (ES+) calculated for C24H24N6O6 492.1757, found 493.2 (M+H+), 515.2 (2M+Na+), 1007.4 (2M+Na+).
In general, two approaches were used to obtain the corresponding m2G phosphoramidite. My first approach involved the synthesis of 5′-O-BzH-2′-O-ACE-6-O-DPC-2-N-methyl-guanosine phosphoramidite (
Specifically, the synthesis was carried out as follows:
3′,5′-O-(1,1,3,3-Tetraisopropyl-1,3-disiloxanediyl)-2-N-methyl-6-O-(diphenylcarba-moyl)guanosine [6]. Compound 5 (1.88 g, 3.8 mmol, 1 eq) was azeotroped with benzene in vacuo overnight. This compound was dissolved in 75 mL of dry pyridine. The suspension was stirred for 30 min to give a clear solution and then cooled to 0° C. 1,3-Dichloro-1,1,3,3-tetraisopropyldisiloxane (TIPDSCl2) (1.34 mL, 4.2 mmol, 1.1 eq) was added dropwise (while stirring) to the cold solution over a period of 1 h. Stirring was continued at room temperature for 12 h. The solvent was evaporated, and the light yellow residue was taken up in CH2Cl2, washed with 5% NaHCO3, and then washed with water. The organic layers were combined and washed with brine, dried over Na2SO4, filtered, and concentrated. The crude product was purified by flash column chromatography on silica gel to yield 6 as a pale yellow solid (2.65 g, 95%). TLC (CH2Cl2:MeOH, 12:1 v/v): Rf=0.69; 1H NMR (CDCl3, 400 MHz) δ (ppm): 1.01-1.09 (m, 24H), 1.24 (br.s, 1H), 1.57 (br.s, 4H), 2.98 (d, J=4.8 Hz, 3H), 3.09 (br.s, 1H), 4.04-4.07 (m, 3H), 4.53 (d, J=4.8 Hz, 1H), 4.71 (t, 1H), 5.06 (br.s, 1H), 5.90 (d, J=1.6 Hz, 1H), 7.18-7.22 (m, 4H), 7.29-7.34 (m, 4H), 7.4-7.42 (m, 2H), 7.8 (s, 1H); 13C NMR (DMSO-d6, 400 MHz) δ (ppm): 12.04, 12.27, 12.46, 12.79, 16.82, 16.86, 16.89, 16.98, 17.09, 17.15, 17.31, 28.17, 61.31, 70.33, 73.11, 81.23, 93.99, 116.26, 127.06, 129.30, 139.70, 141.74, 150.34, 155.16, 155.57, 159.59; ESI-MS (ES+) calculated for C36H50N6O7Si2 734.328, found 735.5 (M+H+), 773.4 (M+K+), 1507.7 (2M+K+).
2′-O-[Bis(2-acetoxyethoxy)methyl]-3′,5′-O-(1,1,3,3-tetraisopropyl-1,3-disiloxanediyl)-2-N-methyl-6-O-(diphenylcarbamoyl)guanosine [7]. Compound 6 (0.75 g, 1 mmol, 1 eq) was dried by azeotropic removal of water with anhydrous dioxane in vacuo overnight and then dissolved in 10 mL of anhydrous 1,4-dioxane to give a clear solution. Pyridinium p-toluenesulfonate (0.1 g, 0.41 mmol, 0.4 eq) and tris(2-acetoxyethoxy)-orthoformate (1.3 mL, 4.7 mmol, 4.6 eq) were then added in the given order to give a clear pale yellow solution. The reaction was stirred for 1 h at room temperature and then 4-(tert-butyldimethylsilyloxy)-3-penten-2-one (0.7 mL, 2.8 mmol, 2.8 eq) was added. The solution was stirred and heated at 55° C. with a condenser for 48 h. The reaction progress was monitored by TLC and showed efficient product conversion. The reaction was quenched with N,N,N′,N′,-tetramethylethylenediamine (TMEDA; 0.1 mL, 0.61 mmol, 0.6 eq) and stirring was continued for another 15 min at room temperature. The crude mixture was evaporated and purified by flash chromatography on silica gel to yield 7 as a pale yellow oil (0.5 g, 55%). TLC (CH2Cl2:MeOH=20:1 and TEA=0.5% v/v): Rf=0.7; 1H NMR (CDCl3, 400 MHz) δ (ppm): 0.98-1.08 (m, 28H), 2.1 (q, 1H), 2.19-2.22 (m, 1H), 2.24 (s, 6H), 2.41 (s, 4H), 3.4 (s, 4H), 4.06-4.12 (m, 5H), 4.44-4.46 (m, 1H), 4.57-4.6 (m, 1H), 6.01 (d, 1H), 7.21-7.25 (m, 4H), 7.32-7.36 (m, 4H), 7.40-7.42 (m, 2H), 8.11 (s, 1H), 9.81 (s, 1H); 13C NMR (CDCl3, 400 MHz) δ (ppm) 12.87, 13.22, 13.29, 13.68, 17.21, 17.30, 17.38, 17.57, 17.64, 17.71, 28.62, 45.99, 57.64, 61.72, 70.77, 75.07, 82.48, 89.43, 118.05, 121.22, 122.08, 127.86, 129.48, 129.59, 142.12, 150.66, 154.27, 154.83, 156.32, 163.59; ESI-MS (ES+) calculated for C45H64N6O13Si2 952.407, found 953.4 (M+H+), 975.5 (M+Na+).
2′-O-[Bis(2-acetoxyethoxy)methyl]-2-N-methyl-6-O-(diphenylcarbamoyl)guanosine [8]. Acetonitrile (3 mL), TMEDA (0.76 mL, 5.2 mmol, 10 eq) and HF (48% aq stock solution, 0.12 mL, 3.15 mmol, 6 eq) were added slowly via syringe to a 25 mL round-bottom flask at 0° C. The HF/TMEDA mixture was stirred at 0° C. for 15 min and then transferred to a clear solution of 7 (0.5 g, 0.53 mmol, 1 eq, in 3 mL of acetonitrile) at 0° C. dropwise over 5 min by cannula. The resulting light yellow solution was stirred at 0° C. for 0.5 h and then at room temperature for 3 h. The solvent was evaporated and the crude product was purified by flash chromatography on silica gel with 0.5% TMEDA to yield 8 as yellow oil (0.25 g, 70%). TLC (CH2Cl2:MeOH=20:1 and TEA=0.5% v/v): Rf=0.3; 1H NMR (CDCl3, 400 MHz 2.06-2.15 (m, 6H), 3.05-3.15 (m, 1H), 3.4 (s, 1H), 3.63-3.7 (m, 1H), 3.75-3.79 (m, 4H), 3.79-3.81 (d, 3H), 4.05-4.15 (m, 1H), 4.18-4.25 (m, 4H), 4.25-4.3 (m, 1H), 4.31-4.4 (m, 1H), 4.5 (m, 1H), 5.05-5.12 (m, 1H), 6.01 (d, 1H), 7.21-7.25 (m, 4H), 7.32-7.36 (m, 4H), 7.40-7.42 (m, 2H), 8.11 (s, 1H), 9.71 (s, 1H); ESI-MS (ES+) calculated for C33H38N6O12 710.255, found 711.1 (M+H+), 733.2 (M+Na+), 749.2 (M+K+).
5′-O-[Benzhydryloxybis(trimethylsilyloxy)silyl]-2′-O-[Bis(2-acetoxyethoxy)methyl]-2-N-methyl-6-O-(diphenylcarbamoyl)guanosine [9]. Solution A was prepared by adding diisopropylamine (0.01 mL, 0.07 mmol, 1 eq) dropwise to benzhydryloxybis(trimethylsiloxy)silyl chloride (BzHCl; 0.07 mL, 0.17 mmol, 2.5 eq) in 2 mL of anhydrous CH2Cl2 at 0° C. Solution B was made by adding diisopropylamine (0.01 mL, 0.07 mmol, 1 eq) dropwise to a solution of 8 (50 mg, 0.07 mmol, 1 eq, in 2 mL of anhydrous CH2Cl2) and cooling the resulting mixture to 0° C. Solution A (0.6 mL, 0.5 eq) was added to solution B dropwise, and thereafter every 20 min, 0.3 eq aliquots were added. Reaction was stirred for 3 h at 0° C. The reaction was quenched with 5% NaHCO3 and extracted with CH2Cl2. The organic layer was washed with brine, dried over Na2SO4, concentrated, and purified by silica gel flash chromatography to yield 9 as pale yellow oil in 91% yield (66 mg). TLC (CH2Cl2:MeOH=20:1 and TEA=1% v/v): Rf=0.4; 1H NMR (CDCl3, 400 MHz) δ (ppm): 0.02-0.2 (m, 18H), 1.33 (t, 6H), 2.03 (s, 4H), 3.04 (m, 4H), 3.3 (m, 1H), 3.4 (d, J=5.6 Hz, 3H), 3.74-3.76 (m, 1H), 3.78-3.84 (m, 1H), 4.05 (t, 1H), 4.15 (m, 1H), 4.23 (m, 1H), 4.35 (br.s, 1H), 5.8-6.01 (m, 2H), 7.15-7.46 (m, 20H), 8.21 (s, 1H), 9.79 (s, 1H); 13C NMR (CDC3, 400 MHz) δ (ppm): 1.27, 1.37, 1.46, 20.82, 28.26, 45.96, 60.96, 62.8, 65.16, 71.30, 75.42, 76.17, 85.02, 88.84, 121.51, 126.23, 126.34, 126.44, 126.52, 126.92, 127.02, 127.09, 127.13, 127.19, 127.49, 128.02, 128.12, 128.18, 128.23, 128.43, 129.15, 141.78, 142.22, 143.82, 143.89, 144.08, 144.22, 150.44, 154.24, 154.43, 155.91, 163.39; ESI-MS (ES+) calculated for C52H66N6O15Si3 1098.389, found 1099.5 (M+H+).
5′-O-[Benzhydryloxybis(trimethylsilyloxy)silyl]-2′-O-[Bis(2-acetoxyethoxy)methyl]-2-N-methyl-6-O-(diphenylcarbamoyl)guanosine-3′-(methyl-N,N-diisopropyl)phos-phoramidite [10]. Compound 9 (0.08 g, 0.07 mmol, 1.0 eq) was dissolved in 2 mL of anhydrous CH2Cl2 at room temperature under Ar atmosphere. To the stirring solution, 1H-tetrazole (0.01 g, 0.07 mmol, 1.0 eq) dissolved in diisopropylamine (0.05 mL) was added. After stirring the solution for ˜2 min, the methyl tetraisopropyl phosphoramidite (0.06 mL, 0.2 mmol, 2.8 eq) was added dropwise and the reaction was stirred overnight. The solution initially appeared as a cloudy mixture. The mixture became a pale yellow clear solution after 0.5 h. After 16 h, the TLC showed proper product conversion. The reaction was quenched with 5% NaHCO3 and extracted with CH2Cl2. The organic layer was further washed with saturated NaCl and dried over Na2SO4. The concentrated product was purified on silica gel with 2% TEA in 20:1 mixture of CH2Cl2: MeOH to afford 10 as colorless oil (0.07 g) in 76% yield. TLC (CH2Cl2:MeOH=20:1 and TEA=2% v/v): Rf=0.48; 1H NMR (400 MHz, CD2Cl2) δ (ppm): 0.03-0.06 (m, 60H), 1.12-1.26 (m, 22H), 1.42 (t, 12H), 3.25-3.62 (m, 24H), 5.61 (s, 2H), 5.95 (t, 4H), 7.19-7.37 (m, 40H); 31P NMR (400 MHz, CD2Cl2): δ (ppm): (mixture of diastereomers) 135.35, 150.58; ESI-MS (ES+) calculated for C59H82N7O16PSi3 1259.486, found 1260.6 (M+H+), 1298.5 (M+K+).
In general, since our main goal was to synthesize enough modified RNA for biophysical and biochemical studies, the phosphoramidite was needed in sufficient quantities (>100 mg). Therefore, a different approach was taken in which the phosphoramidite was generated using 5′-O-DMT-2′-O-TOM chemistry.17 The first step involved the reaction between DMT-Cl and 5′-OH of compound 5 to yield compound 11 (
In our hands, compound 5 has lead to higher yields in the m2G phosphoramidite synthesis than the methods reported previously.17, 20 DPC protection at the O6-position enhanced solubility of the m2G nucleoside in solvents used during the phosphoramidite synthesis. It also protected the O6-position from side reactions. The synthesis could be performed on a reasonably high scale to produce sufficient amounts of amidite 13 for multiple couplings.
Specifically, the synthesis was carried out as follows:
5′-O-(4,4′-Dimethoxytrityl)-2-N-methyl-6-O-(diphenylcarbamoyl)guanosine [11]. Compound 5 (0.51 g, 1.05 mmol, 1.0 eq) and 4,4′-dimethoxytritylchloride (0.39 g, 1.14 mmol, 1.09 eq) were azeotroped three times with toluene for ˜15 h. To the dried compound 5, anhydrous pyridine (5 mL) was added. The mixture was stirred at room temperature under Ar atmosphere for 4 h. 4-Dimethylaminopyridine (0.09 g, 0.7 mmol, 0.7 eq) was subsequently added and stirring was continued for 17 h. The reaction was quenched with methanol (1 mL) and evaporated to dryness. The crude residue was dissolved in 50 mL of dichloromethane and washed with 5% sodium bicarbonate followed by saturated sodium chloride. The organic layer was dried over sodium sulfate and filtered. The product was then purified via silica gel chromatography using a solvent mixture of 90% dichloromethane, 9% methanol, 1% triethylamine to give 11 as a light yellow crystalline solid (0.56 g, 67%). TLC (CH2Cl2:MeOH, 9:1 v/v): Rf=0.4; 1H NMR (CD3OD, 400 MHz) 2.71 (br.s, 1H), 2.98-3.03 (q, 1H), 3.21 (d, J=3.2 Hz, 3H), 3.25-3.27 (m, 1H), 3.29-3.32 (m, 1H), 3.60 (d, J=4.8 Hz, 6H), 3.66 (m, 1H), 4.07-4.10 (m, 1H), 4.45 (m, 1H), 4.83 (m, 1H), 5.87 (d, J=4.8 Hz, 1H), 6.64-6.69 (m, 5H), 7.05-7.38 (m, 18H), 8.0 (s, 1H); 13C NMR ((CD3)2SO, 500 MHz) 28.8, 55.6, 72.2, 74.9, 82.3, 85.3, 87.7, 113.8, 114.0, 126.3, 127.8, 128.5, 128.7, 129.1, 129.2, 129.3, 129.9, 130.2, 130.4, 131.2, 141.2, 149.2, 159.9; ESI-MS (ES+) calculated for C45H42N6O8 794.3064, found 795.7 (M+H+), 303.4 ([(MeO)2Tr]+).
5′-O-(4,4′-Dimethoxytrityl)-2′-O-[[(triisopropylsillyl)oxy]methyl]-2-N-methyl-6-O-(diphenylcarbamoyl)guanosine [12]. Di-tert-butyltindichloride (0.26 g, 0.846 mmol, 1.2 eq) was added to a solution of dry 1,2-dichloroethane (6.5 mL) containing compound 11 (0.56 g, 0.705 mmol, 1.0 eq) and ethyldiisopropylamine (0.36 mL, 2.82 mmol, 4.0 eq). The reaction mixture was heated to 70° C. for 15 min under reflux conditions. Then, the mixture was allowed to cool to room temperature. Upon cooling down, the mixture became cloudy and light brown in color. The crude reaction mixture was then stirred with [(triisopropylsilyl)oxy]methylchloride (0.18 mL, 0.776 mmol, 1.1 eq) for 3 h at room temperature. After 3 h, the mixture was evaporated to dryness. The resulting crude residue was dissolved in 20 mL of dichloromethane and washed with saturated sodium bicarbonate followed by saturated sodium chloride. The organic layer was dried over sodium sulfate and filtered. The product was then purified via silica gel column chromatography using a solvent mixture of dichloromethane: methanol (20:1) and triethylamine (0.5%) to give 12 as a light yellow oil (0.49 g, 70%). TLC (CH2Cl2:MeOH, 9:1 v/v): Rf=0.7; 1H NMR (CD3OD, 400 MHz) 0.89-1.05 (m, 18H), 1.25-1.3 (m, 3H), 2.79-2.8 (m, 7H), 3.1 (br.s, 1H), 3.3-3.5 (m, 2H), 3.70 (d, J=4.8 Hz, 3H), 4.15-4.25 (m, 1H), 4.65-4.7 (m, 1H), 4.85 (s, 2H), 5.05-5.15 (m, 1H), 6.1 (d, J=5 Hz, 1H), 6.79-6.83 (m, 5H), 7.17-7.5 (m, 18H), 8.05 (s, 1H), ESI-MS (ES+) calculated for C55H64N6O9Si 980.4504. found 981.9 (M+H+), 1003.9 (M+Na+), 1019.9 (M+K+)
5′-O-(4,4′-Dimethoxytrityl)-2′-O-[[(triisopropylsilyl)oxy]methyl]-2-N-methyl-6-O-(diphenylcarbamoyl)guanosine 3′-(2-cyanoethyldiisopropylphosphoramidite) [13]. Compound 12 (0.25 g, 0.25 mmol, 1.0 eq) was dried extensively under vacuum. Then, it was dissolved in 5 mL of anhydrous dichloromethane. Next, N,N-diisopropylethylamine (0.3 mL, 2.5 mmol, 10 eq) and 2-cyanoethyldiisopropylchlorophosphoramidite (0.08 mL, 0.38 mmol, 1.5 eq) were added and the mixture was stirred for 2 h at room temperature. The reaction was quenched with 5% aqueous sodium bicarbonate, and then it was extracted with 2×50 mL of dichloromethane. Combined extracts were dried over anhydrous sodium sulfate and evaporated. The crude mixture was purified by silica gel column chromatography (hexane:ethyl acetate, 3:1 and triethylamine, 0.5%) to yield 13 as a white form (0.285 g, 95%). TLC (hexane:EtOAc:Et3N=75%:24.5%:0.5%): Rf=0.23; 1H NMR ((CD3)2CO, 400 MHz) (mixture of diastereoisomers) 0.89-1.05 (2 m, 60H), 1.18-1.30 (2 m, 10H), 1.45 (t, 4H), 2.49 (br.s, 2H), 2.79-2.84 (m, 8H), 3.39-3.41 (m, 2H), 3.66-3.75 (m, 14H), 4.17-4.19 (m, 2H), 4.69 (m, 2H), 5.12-5.14 (m, 8H), 6.11 (d, J=5.2 Hz, 2H), 6.79-6.83 (m, 10H), 7.17-7.50 (2 m, 36H), 8.04 (s, 2H); 13C NMR ((CD3)2CO, 400 MHz) 12.56, 18.04, 18.08, 20.7, 20.75, 24.76, 24.82, 24.89, 24.95, 28.97, 43.82, 43.91, 43.96, 44.06, 55.45, 59.0, 59.16, 59.89, 60.02, 64.39, 72.59, 84.4, 84.7, 87.14, 87.71, 90.03, 90.36, 113.86, 127.54, 128.54, 128.58, 128.91, 128.98, 129.91, 130.85, 130.93, 130.99, 136.57, 136.69, 143.38, 145.96, 151.43, 157.33, 159.58, 160.82, 206.15; 31P NMR ((CD3)2CO, 400 MHz) (mixture of diastereoisomers) 150.96, 151.14; ESI-MS (ES+) calculated for C64H81N8O10PSi 1180.5583. found 1181.5 (M+H+), 1203.5 (M+Na+), 1219.4 (M+K+); High resolution ESI-MS (ES+) calculated for C64H81N8O10PSi 1180.5583. found 1181.5634 (M+H+), 1203.5439 (M+Na+), 1219.5358 (M+K+)
970 Loop Model Constructs
Chemical synthesis of 970 loop model constructs. Four RNA analogues representing the 970 stem-loop region (h31) of E. coli 16S rRNA, were chemically synthesized at the W. M. Keck Foundation at Yale University, New Haven, Conn., USA (
For RNAs containing 2-N-methyl-guanosine, 50 μmoles from the corresponding phosphoramidite were provided. The 5-methylcytidine phosphoramidite was purchased from Glen Research along with the standard A, U, C, and G amidites. The numbering system is based on the full-length E. coli rRNA sequence.21 A G-C base pair was added at the end of the stems (denoted by lower case g-c) to stabilize the hairpin structure. Residues in all four constructs are numbered from g1 to c18 for the ends and U960 through A975 for the component representing the natural E. coli h31 sequence. Two h31 RNAs (ECh31UNMOD and ECh31M5C) were obtained using commercial amidites. The other two h31 analogues (ECh31M2G and ECh31WT) were synthesized using the 5′-O-DMT-2′-O-TOM-6-O-DPC-2-N-methylguanosine phosphoramidite along with commercially available amidites. The doubly modified h31 analogue (ECh31WT) represents the wild-type sequence of E. coli 16S rRNA helix 31.
Post-synthetic processing of RNA constructs. Upon completion of coupling on an automated synthesizer, the CPG-bound RNA was cleaved from the solid support and deprotected with 1:3 (v/v) EtOH/NH4OH and TBAF (tetrabutylammonium fluoride solution, 1 M in THF) as described in the literature.8, 18 These steps will remove the 6-O-DPC and 2′-TOM protections on the m2G modified nucleoside simultaneously. The 2′-silyl protections were then removed either by Et3N.3HF or TBAF (tetrabutylammonium fluoride solution, 1M in THF) as described in the literature.8, 18 Basically, 1 mL of TBAF was added to the dried oligo and vortexed. The modified RNAs containing 2′-TOM protecting groups were less soluble than the RNAs containing only 2′-TBDMS protections. Therefore the 2′-TOM-protected RNAs were warmed to 50° C. with shaking for 10 min to completely dissolve the RNA. Then, the solutions were allowed to cool to 35° C. and shaken overnight to attain complete deprotection. The reaction was quenched by adding 1 mL of 1 M Tris.HCl buffer (pH 7.5). This step also removes the 2′-hemiacetals remaining from the 2′-TOM protections in the modified RNAs.
The RNAs were desalted over Poly-Pak II cartridges (Glen Research cat. 60-3100-01) to remove the fluoride ions present in the mixture. To avoid any adverse effects of THF on the RNA binding to the cartridge matrix, the mixture was first dried to about half the original volume to remove THF from the mixture. Then, 1 mL of 0.1 M TEAA (pH 7.0) was added to the mixture making the total volume up to ˜2 mL. Prior to sample introduction, the cartridge was flushed with 4 mL of acetonitrile to swell the resin and to remove any organic impurities. It was then flushed with 4 mL of 2 M TEAA (pH 7.0) which acts as an ion pairing agent to enhance the binding of RNA to the matrix. After loading the RNA-containing mixture onto the cartridge, it was flushed with 6 mL of 0.1 M TEAA (pH 7.0) to remove the salts. Then, the RNA was eluted with 1-2 mL of 50% acetonitrile. It is essential to maintain a flow rate of ˜1-2 drops per second throughout the desalting process in order to obtain a higher efficiency of RNA recovery.
The RNAs were purified by HPLC (see HPLC methods for more details). After HPLC purification, each oligomer was further desalted by ethanol precipitation and dialysis for 3 days against RNase-free, deionized water using a 1000 molecular weight cut-off membrane (Spectra-Por). RNA concentrations were calculated using Beer's law and a single-stranded extinction coefficient (ε) of 176,900 M−1 cm−1.22 The same extinction coefficients were used for guanosine and N2-methylguanosine (1.4×104M−1 cm−1 at pH 7.0) and cytidine and 5-methylcytidine (9.1×103 M−1 cm−1 at pH 7.0). These steps are summarized in
Characterization of RNA constructs. It is quite important to verify that the methyl group of m2G remains intact after carrying out all the RNA synthesis and deprotection steps. The incorporation of m2G residues was first confirmed by MALDI-TOF mass spectrometric analysis of full-length RNA and then by P1 nuclease digestion and calf intestinal phosphatase (CIP) treatment of the RNAs, followed by reverse-phase HPLC analysis of the enzyme digest products. The results are shown in
For the HPLC characterization, retention time (tR) values of the individual nucleoside standards were first obtained as shown in
The above retention time (tR) values (6.7, 9.5, 15.9, 19.2, 18.7, and 12.5 min. for C, U, G, A, m2G, and m5C, respectively) were then used to determine the peaks seen from the enzyme digested h31 RNA samples (
General Procedures for Examples 7-13
RNA sample preparation. The four RNA hairpins used in this study were chemically synthesized at the W. M. Keck Foundation at Yale University, New Haven, Conn., USA. For RNAs containing N2-methylguanosine, 50 μmoles of the corresponding phosphoramidite were provided. The 5-methylcytidine phosphoramidite was purchased from Glen Research. Upon completion of coupling on an automated synthesizer, the CPG-bound RNA was cleaved from the solid support and deprotected with 1:3 (v/v) EtOH/NH4OH and TBAF (tetrabutylammonium fluoride solution, 1 M in THF) as described in the literature.22, 23 The RNAs were desalted over Poly-Pak II cartridges (Glen Research), then purified by HPLC on an XTerra MS C18 column (2.5 μm, 10×50 mm, Waters) in which the eluent was 0.1 M TEAA (triethyl ammonium acetate) buffer, pH 7.0, with a 5-15% linear gradient of acetonitrile over 25 min at a flow rate of 4.0 mL/min. After HPLC purification, each oligomer was further desalted by ethanol precipitation and dialysis for 3 days against RNase-free, deionized water using a 1000 molecular weight cut-off membrane (Spectra-Por). RNA concentrations were calculated using Beer's law and a single-stranded extinction coefficient (c) of 176,900 M−1 cm−1.24 The same extinction coefficients were used for guanosine and N2-methylguanosine (1.4×104 M−1 cm−1 at pH 7.0) and cytidine and 5-methylcytidine (9.1×103 M−1 cm−1 at pH 7.0).
Thermal melting studies. The absorbance versus temperature profiles were obtained on an Aviv 14DS UV-vis spectrophotometer with a five-cuvette thermoelectric controller. Microcuvettes with two different pathlengths, 0.1 and 0.2 cm (60 and 120 μL volumes, respectively), were employed. Each set of measurements was done in triplicate. The buffer used in each experiment contained 15 mM NaCl, 20 mM sodium cacodylate, and 0.5 mM Na2EDTA (pH 7.0) unless otherwise noted. Each oligomer was dissolved in a specific volume to yield an absorbance reading just below 2.0 in a 0.1 cm pathlength cuvette. The RNA concentrations were determined from the absorbance values (260 nm) at 95° C. The absorbance data were collected at 280 nm from 0 to 95° C. with a constant heating rate of 0.5° C./min. Thermodynamic parameters were obtained from the absorbance versus temperature profiles using the MELTWIN v. 3.5 melting curve program.1 This program performs a van't Hoff analysis, assuming a two-state model for the transition between a native and a denatured (random coil) structure of a hairpin.
Circular dichroism studies. CD spectra were obtained on an Applied Photophysics Chirascan circular dichroism spectrometer (220-320 nm) at 25° C. in 15 mM NaCl, 20 mM sodium cacodylate, and 0.5 mM Na2EDTA at pH 7.0 unless otherwise noted. The RNA concentrations were maintained at 2.5-3.0 μM for all CD experiments. Based on the RNA strand concentration, the measured CD spectra were converted to molar ellipticity (Δε),25 which denotes the moles of RNA molecules rather than moles of individual residues present in the sequence.
NMR experiments. The HPLC-purified RNAs (˜150 μM) were further desalted by ethanol precipitation, followed by desalting in two steps: 1) dialysis against double-deionized water in the presence of 0.1 M NaCl and 0.1 mM EDTA for 1 day, and 2) dialysis against double-deionized water for 2 days. All four RNAs were dissolved in 40 mM NaCl, 10 mM sodium phosphate, 0.5 mM Na2EDTA, and 15 μM TSP-d4 (sodium 3-(trimethylsilyl)tetradeuteriopropionate), in 90% H2O and 10% D2O at pH 6.8. The NMR spectra were obtained on a Bruker AVANCE-AQS 700 MHz spectrometer equipped with a 5 mm triple-resonance cryoprobe. All NMR spectra were acquired at 20° C., except for variable temperature experiments that ranged from 5 to 30° C. ID imino proton NMR spectra were acquired for all samples using Digital Quadrature Detection for at least 16,000 data points. The water samples in 9:1 H2O/D2O required additional Watergate solvent suppression pulse schemes to be included in the pulse program. 1D NOE difference spectra included a 500 msec presaturation pulse centered on imino peaks of interest. A reference spectrum was subtracted from the resulting selective saturation spectra to obtain the 1D NOE difference spectra for each construct. For each experiment, 256 scans×10 iterations were acquired in order to improve the signal to noise ratio. The data were further processed with solvent baseline correction, zero-filling one time and 3 Hz of line broadening.
Effect of Modifications on the Stability of Helix 31 Hairpin from E. coli 16S rRNA
Absorbance versus temperature profiles (melting curves) were obtained at pH 7.0 for all four RNA constructs. They were analyzed in terms of ΔG°37, ΔG°50, ΔH°, ΔS°, and melting temperature (Tm),1, 2 Representative normalized UV melting curves of the modified RNAs compared to the unmodified RNA, taken in 15 mM NaCl, 20 mM sodium cacodylate, 0.5 mM Na2EDTA (pH 7.0), are shown in
The curves represent an average of five sets of data at different concentrations of RNA obtained from a five-cuvette thermoelectric controller. The melting curves for the unmodified RNA (ECh31UNMOD, blue line in panels A-C) are compared to those for the modified RNAs (pink lines: (A) ECh31WT, (B) ECh31M2G, and (C) ECh31M5C). All of the melting curves were normalized at 95° C. and absorbance measurements were taken at 260 nm (see materials and methods, section 4.5).
The melting curves are biphasic for all four RNAs (
TABLE 2
Thermodynamic data for ECh31WT, ECh31M5C, ECh31M2G, and
ECh31UNMOD RNA sequences.
ΔG° 50 (kcal/mol)
ΔG° 37 (kcal/mol)
ΔH° (Kcal/mol)
ΔS° (cal/K · mol)
Tm (° C.)
ECh31UNMOD
−0.9a
−2.6 ± 0.1
−44.1 ± 1.0
−133.8 ± 3.0
57
ECh31M5C
−0.6a
−2.2 ± 0.1
−40.5 ± 0.9
−123.3 ± 3.1
55
ECh31M2G
−0.7a
−2.4 ± 0.1
−41.9 ± 1.1
−127.5 ± 3.2
56
ECh31WT
−0.5a
−2.1 ± 0.1
−37.5 ± 2.2
−114.4 ± 5.8
56
The RNA samples were analyzed as five different dilutions per experiment and UV melts were also performed in triplicate for each construct. AU0-AU4 represent profiles corresponding to different dilutions of each RNA taken in 15 mM NaCl, 20 mM sodium cacodylate, 0.5 mM Na2EDTA at pH 7.0. Experiments in K+ buffer (15 mM KCl, 20 mM cacodylic acid, 20 mM Tris [basic form], 0.5 mM Na2EDTA, pH 7.0) gave similar results (Table 3,
TABLE 3
Thermodynamics of the ECh31 WT RNA in Na+ and K+ buffers.
ΔG°37
ΔH°
ΔS°
Tm
(kcal/mol)
(kcal/mol)
(cal/K · mol)
(° C.)
ECh31WT -
−2.13 ± 0.03
−39.37 ± 1.2
−120.08 ± 3.8
54.7
KCl buffer
ECh31WT -
−2.10 ± 0.07
−37.26 ± 1.2
−113.37 ± 3.6
55.5
NaCl buffer
The subtle destabilizing effects of the methylations were somewhat unexpected. In X-ray crystal structures of E. coli 70S ribosomes5 and T. thermophilus 30S ribosomes,6 m2G and m5C are involved in a base-triple stacking interaction with residue 968. One might expect the methyl groups in the modified nucleosides to facilitate stacking interactions;7 however, both m2G and m5C are destabilizing relative to standard nucleotides G and C within the given sequence context. The presence of the h31 methylations might serve another purpose, such as stabilizing the ribosome through hydrophobic interactions with Arg128 of the S9 protein.7 Furthermore, the slight destabilization caused by the base methylation may facilitate base flipping of m2G966, which has been observed in ribosome crystal structures and likely plays an important role in protein synthesis.8 The energetic penalty would then be overcome by contacts with various ribosome components such as 16S rRNA-helices, ribosomal proteins, and tRNA.8 Furthermore, the X-ray crystal structure of the T. thermophilus 70S ribosome complexed with a model mRNA and two tRNAs revealed that the positions of the 16S rRNA P-site nucleotides in the vacant ribosome superimpose well with those in the tRNA-containing complex, with the exception of m22G966.8 Residue m22G966 is flipped out in the crystal structure of the T. thermophilus 70S ribosome containing a model mRNA and two tRNAs (
Effect of Modifications on the Structure of Helix 31 Hairpin from E. coli 16S rRNA
Circular dichroism studies. The CD spectra of the helix 31 analogues were obtained to analyze the effects of modifications on the folded structure (
In
ECh31M5C+ECh31M2G−(2×ECh31UNMOD)=ECh31WT−ECh31UNMOD (1)
difference=ECh31M5C+ECh31M2G−ECh31UNMOD−ECh31WT (2)
As shown in
The CD experiments were repeated for ECh31WT RNA in 35 mM K+ buffer (KCl buffer) and salt concentrations that more closely mimic in vivo protein synthesis conditions10 (25 mM cacodylic acid, 25 mM Tris [basic form], 30 mM KCl, 70 mM NH4Cl, 3 mM MgCl2 at pH 7.0; Mg buffer). The spectra taken in K+ and Mg2+ containing buffers are similar (
1D NMR studies. ID NMR spectroscopy was employed to examine hydrogen-bonding interactions in the four RNA constructs. The signals corresponding to the imino protons can be observed only when those protons are protected from exchange with the bulk solvent (water). That is generally possible when they are involved in hydrogen-bonding interactions. Other types of tertiary structures (including base stacking) may also lead to protection from solvent exchange. Simply by counting the number of imino proton resonances present in the region of 10 to 15 ppm, it is possible to determine the number of base pairs present in the stem region if only standard Watson-Crick base-pairs are present. Additional peaks may arise from non-standard base-pairing interactions such as base mismatches. In order to investigate the stability of the RNA-stem-regions, we performed 1D-experiments at temperatures ranging from 5 to 25° C. The 1 D imino-proton spectra were obtained at variable temperatures for each of the helix 31 RNA constructs (
The variable temperature experiments provided a suitable temperature for NOE difference experiments to be performed. The temperature at which all the imino proton peaks corresponding to the base-pairing interactions of the four RNA constructs was found to be 20° C. Also, this temperature (20° C.) gave rise to minimal effects from the spectral artifacts that would otherwise appear at lower temperatures as evident from the biphasic nature of the UV melting transitions (
Peak assignments of the imino proton spectra were made using ID NOE difference spectroscopy. The corresponding analyses are shown in
The imino proton regions of the 1H NMR spectra of four RNA analogues and their peak assignments based on ID NOE difference spectroscopy are summarized in
All four spectra in
The helix 31 Corresponding to H. sapiens 18S rRNA
The 970 loop of helix 31 (h31) of E. coli 16S rRNA is located near the ribosomal P site and therefore believed to be intimately involved in translation.8, 9, 11 E. coli h31 contains two modified nucleotides, N2-methylguanosine at position 966 (m2G966) and 5-methylcytidine at position 967 (m5C967) as shown in
Stability Studies on the Unmodified Helix 31 Corresponding to H. sapiens 18S rRNA.
Thermal melting studies. Preliminary experiments were performed with the unmodified human analogue (HSh31UNMOD) containing an additional G-C base-pair (denoted by g-c) similar to that of the ECh31UNMOD construct (
TABLE 4
Thermodynamics of the unmodified RNA model constructs
representing E. coli and H. sapiens h31
ΔG°37
ΔH°
ΔS°
Tm
(kcal/mol)
(kcal/mol)
(cal/K · mol)
(° C.)
HSh31UNMOD
−0.6 ± 0.1
−29.4 ± 1.6
−92.8 ± 5.4
44
ECh31UNMOD
−2.6 ± 0.1
−44.1 ± 1.0
−133.8 ± 3.0
57
The HSH31UNMOD analogue was unstable with respect to hairpin formation, as indicated by the relatively low negative value for the free energy (ΔG°37=−0.6 kcal/mol). Also, this value was not very reproducible, possibly due to formation of G quartets by the highly abundant guanine residues in the stem region. In order to alleviate this problem, we tried different buffer conditions used previously in the literature.4, 14, 15 First, we increased the NaCl concentration to 1 M keeping the remaining components constant. Therefore, the buffer contained 1 M NaCl, 20 mM sodium cacodylate, and 0.5 mM EDTA at pH 7.0. In
In another attempt, we added 5 mM MgCl2 to the buffer. The new buffer contained 15 mM NaCl, 20 mM sodium cacodylate, 0.5 mM EDTA, and 5 mM MgCl2 at pH 7.0. The result obtained in the presence of Mg2+ (dashed line) is compared with that obtained under the first set of buffer conditions (solid line) in
Structural Studies on the Unmodified Helix 31 Corresponding to H. sapiens 18S rRNA
Circular dichroism studies. CD experiments were carried out under the standard buffer conditions (15 mM NaCl, 20 mM sodium cacodylate, and 0.5 mM EDTA at pH 7.0). The HSH31UNMOD spectrum has a peak maximum at 270 nm with an increase in peak intensity at the maximum (˜2 ellipticity units) compared to ECh31UNMOD, and a peak minimum at 240 nm and a crossover point at 252 nm. Differences in the CD spectra between the E. coli and H. sapiens RNAs were not surprising, because they have different stem sequences.
MFOLD analysis on the unmodified helix 31 of H. sapiens 18S rRNA. The above observations from UV melting and CD were further supported by MFOLD analysis16 carried out on the given HSH31UNMOD RNA. The free energy data obtained from MFOLD revealed that hairpin formation from the given sequence is relatively unfavorable (
Phylogenetic analysis to reveal the base-pair conservation in the stem region of helix 31. The observed instability of the HSh31UNMOD hairpin raised doubts about its utility as a model construct to represent the human helix 31. Consequently, the requirement for a stable stem region for the study was recognized. In an attempt to determine other possible sequences for the stem region of helix 31, the sequences of rRNAs from a series of organisms were compared (
Stability Studies: An Altered Oligonucleotide Sequence for the Helix 31 of H. sapiens 18S rRNA
The aforementioned phylogenetic analysis revealed several other possible base pairs for the stem region of the H. sapiens model helix 31. It also revealed that replacement of the three consecutive G:U wobble pairs by the secondary possibilities provide a stem region similar to that of the E. coli helix 31 as shown by the construct HSh31ECstem (
Thermal melting studies on the human unmodified helix 31 containing the altered sequence. The absorbance versus temperature profiles were obtained at pH 7.0 in low salt conditions (35 mM Na+) for the new analogue of helix 31 (HSh31ECstem) and analyzed in terms of the melting temperature (Tm), Δ°, ΔS° and ΔG°37. The melting curve for HSH31ECSTEM (green color curve) is biphasic with transitions at 0-35 and 45-80° C. (
A comparison of HSh31UNMOD vs. HSh31ECstem (
TABLE 5
Thermodynamics of the HSh31ECstem RNA as compared
with ECh31UNMOD and HSh31UNMOD RNAs.
ΔG°37
ΔH°
ΔS°
Tm
(kcal/mol)
(kcal/mol)
(cal/K · mol)
(° C.)
HSh31UNMOD
−0.6 ± 0.1
−29.4 ± 1.6
−92.8 ± 5.4
44
HSh31ECstem
−1.8 ± 0.1
−43.1 ± 0.3
−133.1 ± 1.0
51
ECh31UNMOD
−2.6 ± 0.1
−44.1 ± 1.0
−133.8 ± 3.0
57
Structural Studies on the Human Unmodified Helix 31 Containing the Altered Sequence.
Circular dichroism. The CD spectra of the helix 31 analogues show peak maxima around 265 nm and minima around 240 nm, similar to other A-form RNAs (
General Procedures for Examples 15-18
Media and bacterial strains. Cells were grown in LB media (10 g of bactotryptone, 0.5% (5 g) NaCl (instead of 1% in normal media) and 0.5% (5 g) yeast extract in 1 L) as suggested by New England Biolabs (NEB) (Beverly, Mass.). For plates, 18 g (1.8%) of agar was added to 1 L of LB. To make soft or top agar, 14 g (1.4%) of agar was added to 1 L of LB. The E. coli ER2738 strain (New England Biolabs) was used to infect M13 bacteriophage and amplify its population. Its genotype is: F′lacIq Δ(lacZ)M15, proA+B+zzf::Tn10(TetR)/fhuA2, supE, thiΔ(lac-proAB), Δ(hsdMS-mcrB)5, (rk−mk−McrBC−).
Biotinylation of target RNA. The 18 mer wild-type h31 contains m2G966 and m5C967 modified nucleotides. Dinuka Abeydeera (Chow lab) prepared the m2G phosphoramidite and its incorporation into RNA was done at the W. M. Keck Foundation, Yale University, CT. It was deprotected and purified by D. Abeydeera using manufacturer's instructions. The unmodified h31 was purchased from Dharmacon Inc, Lafayette, Colo. and it was deprotected and purified by 18% polyacrylamide denaturing gel (7 M urea, 29:1 acrylamide and bisacrylamide). The 5′-end of RNA was biotinylated as follows. One nmole of RNA oligo was mixed with 5 μl of polynucleotide kinase (PNK, 50 units), 3.5 μl of ATP-γ-S (final concentration, 0.2 mM), 5 μl of 10× polynucleotide kinase buffer and the mixture was incubated at 37° C. for 1.5 h. The PNK enzyme was inactivated by keeping the tubes at 70° C. in a water bath for 15 min. The reaction mixture was dried on speed vac evaporator before carrying out the coupling reaction. Coupling of the phosphorothioate RNA oligo with biotin was done by mixing 45 μl of potassium phosphate (KHPO4), pH 8.0 buffer (final concentration, 90 mM), and 5 μl of NIBH (N-iodoacetyl-N′-biotinylhexyldiamine) (final concentration, 2 mM); then, the reaction was kept at 50° C. in a water bath in the dark for 1 h. The NIBH solution was prepared in dimethyl formamide (DMF) by warming to 50° C. in a water bath for 20 min. It was stored at 4° C. in the dark. The coupled biotinylated product was separated from uncoupled RNA on a denaturing 20% denaturing PAGE gel (7 M urea, 29:1 acrylamide:bisacrylamide). The RNA was recovered from the polyacrylamide gel by electroelution and ethanol precipitation. The molecular weight of product was confirmed by MALDI-TOF mass spectrometry.
Biopanning of rRNA (h31) target. Ph.D.-7® (New England Biolabs, Ipswich, Mass.), a 7 mer library, was used for screening. Before starting the screen, a culture of E. coli ER2738 cells was grown in LB+tetracycline [35 .mu.g/ml] media. Approximately 25 mu.L of Dynabeads (M−280 streptavidin beads—Dynal Biotech, Oslo, Norway) were added to a 0.1 mL PCR tube. Three tubes were used for both modified and unmodified h31 target. The target was run in 2 tubes (identical target) and the control in the 3rd tube. The PCR tubes were placed in a magnetic holder and bead storage buffer was removed. The beads were washed three times with 100 μL of buffer A (0.1 M NaOH, 0.05 M NaCl). During washing, tubes were set on the magnetic holder and the supernatant was removed by pipetting. Beads were then washed once with 100 μL of buffer B (0.1 M NaCl) followed by 1× Fish binding buffer (10 mM Tris-C1, pH 8.0, 1 M NaCl). Fifty pmoles of biotinylated h31 (modified or unmodified) rRNA and 50 μl of 2× Fish binding buffer were added together with ddH2O to give 100 μl total volume, and the mixture was incubated for ½ hr at RT. At the same time, another set of beads that were washed with buffer A and buffer B, were then washed with RNA/phage washing buffer (10 mM Tris-C1, pH 7.5, 10 mM MgCl2, 150 mM NaCl, 1 mM DTT). Ten microliters of phage library (2×1011 phage particles) were added to the beads with 90 μl RNA/phage binding buffer and incubated for ½ hr at RT. The supernatant was taken out, which comprises the pre-screened phage library. This library was titered to quantify the phage concentration. This pre-screening step was carried out to remove phage with non-specific binding to beads and tubes. The tubes with beads in which target RNA was bound were washed twice with 100 μl of RNA/phage binding buffer to remove unbound biotinylated RNA. The pre-screened phage library was stored in RNA/phage binding buffer. Approximately 2×1011/15 μl pre-screened phage library, 8 μl of E. c tRNAPhe (30 pmole), 10 μl of 10×RNA/phage binding buffer, 67 μl of DEPC (diethylpyrocarbonate) treated water was added to h31 RNA-bound magnetic beads and incubated at room temperature for ½ hr. Thirty pmoles of tRNAPhe was added in every round as a competitor so that any non-specific RNA binding phage could be removed. Following incubation, the unbound phages were removed by washing the tubes with 200 μl of RNA/Phage washing buffer containing 0.1% Tween-20 (Fisher Scientific) 12 times as shown in Table 7. During washing, the tubes were kept in the magnetic holder and incubated for one minute after the addition of washing buffer. After washing was done, the bound phage were eluted from the beads non-specifically by incubation with 100 μl of elution buffer (0.2 M glycine-HCl, pH 2.2, 1 mg/ml BSA) for 9 min followed by mixing with 15 μl of neutralization buffer (1 M Tris-HCl, pH 9.1). The eluant represents the unamplified phage pool, which was amplified by infecting E. coli cells (described in next section). This step of enrichment ensured that the phage quantity was sufficient for the next round of selection. After the first round, the amplified phage library was not prescreened against magnetic beads/tubes before starting the round. The stringency of washing was increased by changing the number of washes and amount of Tween-20 in consecutive rounds (Table 7). The beads were washed 16 times in the second round and 24 times in the round 3 with buffer containing 0.3% Tween-20. The concentration of Tween-20 was increased to 0.5% in the fourth round with the same washing conditions as round 3.
Amplification of phage. The overnight culture of ER2738 cells was diluted to 1:100 in 20 mL of LB/Tet medium. Unamplified phage (10 μl) was added to the diluted cells and allowed to grow for 4.5 h at 37° C. in an air shaker. After transferring the culture into an Oakridge tube, it was centrifuged for 10 min at 10,000×g at 4° C. Almost two thirds of the supernatant was transferred into another tube and ⅙ volume of 20% PEG (polyethylene glycol)/2.5 M NaCl was added to precipitate the phage particles. The tubes was kept overnight at 4° C. and on the following day, it was centrifuged at 10,000×g for 15 min at 4° C. After removing the supernatant, the pellet was dissolved in 1 mL TBS buffer (50 mM Tris-Cl, pH 7.5, 150 mM NaCl). The pellet was completely dissolved by vortexing and transferred to a 1.7 ml microcentrifuge tube. Again, ⅙ volume of 20% PEG/2.5 M NaCl was added and the solution was kept on ice for 45 min. The phage particles were pelleted by centrifuging for 5 min at 10,000×g. Finally, the pellet containing the amplified phage was dissolved in 100 μl of TBS buffer and stored at 4° C. The number of phage particles was determined by a plaque assay.
Plaque assay. Phage were grown on LB-Xgal/IPTG/Tet plates. Due to the presence of the lacZ gene on the phage plasmid, the plaques turn blue in the presence of Xgal/IPTG. The plates were pre-warmed at 37 C. The low melting agar was prepared and aliquoted into 3 mL portions in 13 mM sterile tubes. The tubes with low melting agar were stored in a 50.degree. C. water bath until use. Serial dilutions of both amplified and unamplified phage was done. For unamplified phage, 10 μl of eluted phage were diluted up to 10−5, for amplified phage, the dilution was made up to 10−11. Next, 200 μL of 1:80 dilutions of overnight culture of ER2738 cells were added to each 0.7 mL microcentrifuge tube. Finally, 10 μL of diluted phage were added to the 0.7 mL microcentrifuge tube containing diluted ER2738 cells. After mixing serially diluted phage with ER2738 cells, they were kept at room temperature for 1-3 minutes. The warm top agar was mixed with phage infected E. coli, vortexed briefly, and immediately poured on top of the pre-warmed LB/X-gal/IPTG/Tet plate. The plates were kept for 10-15 minutes for complete solidification and were incubated at 37° C. incubator for about 15-18 hrs. The next day, blue plaques of phage were observed. For each dilution, the number was counted from each plate and plaque-forming units (pfu) were determined by multiplying the dilution factor by the number of colonies. The plaque assay for the unamplified phage was done in a similar way using only five dilutions from 10−1 to 10−5. From unamplified phage plaque assay, we can determine the input and output ratio (Tables 6, 8, and 10). Plaque assays were performed before and after each round of selections.
Sequencing of phage clones. Phage were amplified and sequenced at the end of rounds three and four. First, the blue phage plaques were removed from LB/Tet/IPTG/X-Gal plate and dipped into 10 .mu.1 of PCR master mix. The region of peptide in the plasmid was amplified using the appropriate primers (bind in the flanking region of peptide) (Table 6) with the following conditions: denaturation (5 min, 95° C.); cycle: denaturation (15 sec, 95° C.); annealing (15 sec, 55° C.); polymerization (15 sec, 72° C.). This cycle was repeated 29 times and the final polymerization step was carried out for 5 minutes. The amplification step was carried out in 96-well plate (thin wall PCR plate, GENE Mate, Kaysville, Utah). The amplified PCR product was cleaned up using a robotic program. The program was designed in this way: The PCR product (10 mu.1) was mixed with 18 mu.1 of magnetic beads (Agencore® Ampure® beads, Agencourt Bioscience Corporation, Beverly, Mass.) in 96-well PCR plate (Thin wall PCR plate, GENE Mate, Kaysville, Utah) and incubated for 5 min to allow for binding. The plate was then transferred to the 96-well magnetic plate (Agencourt SPRIPIate® 96R—Ring Magnet Agencourt Bioscience Corporation, Beverly, Mass.) and kept for 5 min. The DNA is bound to the magnetic beads and which adhere to the side of tube so that the buffers and reagents from PCR (dNTP, buffers, Ampli Taq polymerase) can be removed. One hundred microliters of 70% ethanol were added, incubated for 5 min, and then removed. This step was repeated twice. Finally, in the elution step, 100 μl of water was added to the beads and the plate was transferred to the non-magnetic holder. The beads were mixed well with water and incubated for 10 min so that DNA would be eluted from the beads. The plate was again transferred to the 96-well magnetic plate and incubated for 10 min to separate the magnetic beads from DNA. The DNA (at the bottom of tube) was transferred to a new 96-well plate. All of these steps were performed on the Biomek® FX instrument, Beckman Coulter Inc. Fullerton, Calif. Finally sequencing reactions were performed by using the primers shown in Table 6.
TABLE 6
Primer sequences used for PCR and sequencing of peptides are
shown.
Primers
Description
Sequence (5′ to 3′)
PCR M13 PD1
Forward primer to amplify peptide
GCA AGC TGA TAA ACC GAT ACA AT
region n M13 phage
PCR M13 PD2
Reverse primer to amplify peptide
CCC TCA TAG TTA GCG TAA CG
region in M13 phage
M13 pd3 (700)
Primer to sequence petide region
TCC AGA CGT TAG TAA ATG AA
(700 channel primer)
M13 pd3 (800)
Primer to sequence the peptide
TCC AGA CGT TAG TAA ATG AA
region (800 channel primer)
Target Preparation
The 18-nucleotide wild-type and unmodified h31 constructs were used as bait for peptide screening in phage display (
Screening of Phage Display Peptide Library Using Modified h31 as a Target
Two identical targets of h31 (T1h31, T2h31) and one control with no target (beads only) were freshly prepared for each round of selection. Pre-washed, streptavidin-coated magnetic beads (M−280) were mixed with 5′-biotinylated h31 RNA and allowed to bind in polypropylene PCR tubes at room temperature. The peptide library (Ph.D.-7™, 10 .mu.1, 2×1013 pfu/ml) was pre-selected against the beads to remove non-specifically binding phage. The supernatant (unbound phage with low affinity for beads and plastic PCR tubes) was titered to quantify the number of phage. After the removal of excess unbound RNA from the RNA-streptavidin complex, about 2×1011 M13 phage particles from the pre-selected library were added to RNA-streptavidin complex and incubated with TNMD (10 mM Tris-C1, pH 7.5, 50 mM NaCl, 10 mM MgCl2 and 1 mM DTT) buffer. The unbound and weakly bound phage were removed by washing with the same buffer. The bound phage were then eluted and amplified for the next rounds of screening by infecting into a specific E. coli strain. The number of washes and concentration of detergent (Tween-20) were increased in the subsequent rounds of selection to remove any weakly bound and non-specific peptides (Table 7). In each round, 30 pmole of free tRNA was added as a competitor to remove non-specific RNA-binding peptides. In the third round, the biopanning was carried out with and without free unmodified h31 as a counter-selection method. This strategy was used to remove peptides with affinity to unmodified h31 and retain those with affinity for modified h31. The number of bound phage increased with each round of selections, indicating successful enrichment of target-specific peptides (Table 8).
A random peptide library was screened against modified h31 (970 loop) of 16S rRNA to identify peptide ligands. The library was pre-screened to remove non-specific peptides that have higher affinity to beads and plasticware so that they would not get enriched in further rounds of selection. In every round of selection, tRNA was added as a competitor that would help to bypass non-specific RNA-binding peptides. This step helps to obtain target-specific peptides. The number of bound phage was increased with each round of selection (Table 8), indicating the successful enrichment of target-specific peptides. The selection procedure was validated by screening the library against streptavidin beads without adding any target. The number of peptides having-HPQ motifs, which are known binders for streptavidin, were about 65% of the total peptides in the third round and their number increased to approximately 85% in the fourth round of selection (
TABLE 7
Biopanning conditions using wild-type h31 RNA as a target
Cycle no.
Cycle 1
Cycle 2
Cycle 3
No. of washes (200 μl/wash)
12
18
24
Tween-20
0.10%
0.10%
0.30%
Target RNA (unmodified h31)
50 pmole
50 pmole
30 pmole
Competitor RNA (tRNA)
30 pmole
30 pmole
30 pmole
Competitor RNA (tRNA +
—
—
30 pmole, each
unmodified h31)
In the third round of selection with modified h31 as the target, specific peptides were isolated by using the unmodified h31 as a counter-selection agent. The counter-selection was designed to isolate peptides that have higher affinity to modified nucleotides or regions of h31 than to unmodified h31. Based upon sequence analysis, peptides having-TLW- and -VRP motifs were found in the screens using modified h31 as a target with and without counter-selection against unmodified h31. These peptides are expected to display specific binding to modified h31 and interact with residues m2G966 and m5C967. Out of the five major peptides selected for further study, three of them (DIRTQRE (SEQ ID NO: 6), CVRPFAL (SEQ ID NO: 4), FVRPFAL (SEQ ID NO: 7)) contain arginine at the third position of the seven-amino-acid peptide. The presence of R and Q might enhance interactions with the phosphodiester backbone. Two other peptides (TLWDLIP (SEQ ID NO: 3) and TYLPWPA (SEQ ID NO: 2)) contain aromatic tryptophan and tyrosine residues, which might intercalate with nucleobases of h31.
Peptide clones were sequenced after completion of the third round of screening. For each target, 100 plaques (peptide-bearing phage) were sequenced, so altogether for modified h31 target, 300 clones (including with and without counter-selections) were sequenced. The sequences were analyzed by RELIC software, which is a bioinformatics server for combinatorial peptide analysis (74). The peptides obtained repeatedly in the isolated sequences were TLWDLIP (SEQ ID NO: 3), TYLPWPA (SEQ ID NO: 2), ATPLWLK (SEQ ID NO: 5), DIRTQRE (SEQ ID NO: 6), and FVRPFAL (SEQ ID NO: 7) (
TABLE 8
Plaque-forming titration units (pfu) against
modiifed h31 in each rounds of screening
Rounds
Input PFU
Output PFU
% yield
Pre-screen with beads
2.0 × 1011
2.5 × 1010
0.0125
I
2.8 × 1011
2.2 × 106
0.08 × 10−4
II
2.5 × 1011
4.3 × 106
0.17 × 10−4
III
2.2 × 1011
3.1 × 106
0.14 × 10−4
Screening of Peptides by Using Unmodified h31 as a Target
A random peptide library was screened against unmodified h31 (970 loop) of 16S rRNA to identify peptide ligands. The library was pre-screened to remove non-specific peptides that have higher affinity to beads and plasticware so that they would not get enriched in further rounds of selection. In every round of selection, tRNA was added as a competitor that would help to bypass non-specific RNA-binding peptides. This step helps to obtain target-specific peptides. The number of bound phage was increased with each round of selection (Table 10), indicating the successful enrichment of target-specific peptides. The selection procedure was validated by screening the library against streptavidin beads without adding any target. The number of peptides having-HPQ motifs, which are known binders for streptavidin (75), were about 65% of the total peptides in the third round and their number increased to approximately 85% in the fourth round of selection (
We wanted to determine if any common peptide sequences (motifs) would emerge from screening both modified and unmodified h31. The 5′-biotinylated unmodified h31 was used as the target and the selection conditions were similar to those used for modified h31 (Table 9). The number of bound phage increased with each round of selection, indicating successful enrichment of target-specific peptides (Table 10). Peptides were sequenced after the third and fourth round of screening. After analyzing the peptide sequences, two major peptides (HHHPPLA and KPFHNST) were the most abundant (
TABLE 9
Biopanning conditions using unmodified h31 RNA as a target
Cycle no.
Cycle 1
Cycle 2
Cycle 3
Cycle 4
No. of washes
12
18
24
24
(200 μl/wash)
Tween-20
0.10%
0.10%
0.30%
0.50%
Target RNA
50 pmole
50 pmole
30 pmole
30 pmole
(unmodified h31)
Competitor RNA
30 pmole
30 pmole
30 pmole
30 pmole
(tRNA)
TABLE 10
Plaque-forming titration units (pfu) against
unmodiifed h31 in each rounds of screening
Rounds
Input PFU
Output PFU
% of yield
I
2.1 × 1011
3.2 × 105
0.015 × 10−4
II
3.6 × 1011
4.3 × 106
0.12 × 10−4
III
2.3 × 1012
5.2 × 107
0.22 × 10−4
IV
2.5 × 1011
2.6 × 106
0.010 × 10−4
In control experiments, peptides were isolated from screening against streptavidin beads. The conditions used for screening and total input and output ratios of phage are shown in Tables 9 and 10, respectively. Sequence analysis showed a consensus sequence with the conserved HPQ motif (
Screening with unmodified h31 revealed two major peptides, HHHPPLA (SEQ ID NO: 8) and KPFHNST (SEQ ID NO: 9) in round 3. They are mostly polar and rich in histidine residues. The —HHP or —HPP motifs were also seen in some other peptide sequences (
TABLE 11
Biopanning conditions using beads (no target)
Cycle no.
Cycle 1
Cycle 2
Cycle 3
Cycle 4
No. of washes
12
18
24
24
(200 μl/wash)
Tween-20
0.10%
0.10%
0.30%
0.50%
Target RNA
—
—
—
—
Competitor RNA
30 pmole
30 pmole
30 pmole
30 pmole
(tRNA)
TABLE 12
Plaque-forming titration units (pfu) against beads (no target)
Rounds
Input PFU
Output PFU
% of yield
I
2.0 × 1011
TNTC up to 10−5 dilution
—
II
2.7 × 1011
Lawn up to 10−5 dilution
—
III
2.1 × 1012
Lawn up to 10−5 dilution
—
IV
3.1 × 1011
1.0 × 107
0.32 × 10−4
(TNTC—too many too count)
Coupled in vitro Transcription-Translation Inhibition Assay
Peptides with high frequency in the screening against wild-type h31 were synthesized. The peptides (DIRTQRE (SEQ ID NO: 6), CVRPFAL (SEQ ID NO: 4), FVRPFAL (SEQ ID NO: 7), TLWDLIP (SEQ ID NO: 3) and TYLPWPA (SEQ ID NO: 2)), were synthesized and their sequences were determined from the phage display experiments. The inhibitory effects of these peptides on cellular processes were determined by in vitro coupled transcription-translation inhibition assay. The PURExpress™ in vitro protein synthesis kit # E6800S from New England Biolabs (NEB) was used for this purpose. This kit contains all of the necessary components for the transcription and translation, except for the DNA template. The amounts of reagents from the kit were added according to the NEB manual. We used a DNA template for GFP (pRSETEmGFP plasmid) at a concentration of 10 μg/ml in a 15 μl of reaction volume. Different concentrations of peptides were added, ranging from 300 μM to 2 mM. The DNA template was added only after mixing of the peptides or streptomycin so that they can bind to their target region. For the control, streptomycin was added at a final concentration of 300 μM. The reaction was incubated in 384-well, Costar, clear-well, black plates and in situ incubated at 37° C. in the fluorometer. The amount of GFP translation was monitored at different intervals of time from 0 min to 2 h by fluorescence (excitation at 487 nm, emission at 509 nm) using a Gemini XPS microplate spectrofluorometer, (Molecular Devices).
A cell-free translation assay was used to test the inhibitory effects of the peptides on protein synthesis. The pRSETEmGFP plasmid that was used as template has an EmGFP gene under control of the T7 promoter (
From in vitro protein translation inhibition assays, CVRPFAL (SEQ ID NO: 4) and FVRPFAL (SEQ ID NO: 7) showed strong inhibitory effects as compared to others. They showed similar level of inhibition, which could be due to the presence of a common motif. They are different only in first amino acid position. DIRTQRE (SEQ ID NO: 6) showed the least inhibitory effect. The order of translation inhibition by peptides (from high to low) is as follows: CVRPFAL (SEQ ID NO: 4), FVRPFAL (SEQ ID NO: 7)>TLWDLIP (SEQ ID NO: 3)>TYLPWPA (SEQ ID NO: 2)>DIRTQRE (SEQ ID NO: 6). Concentration-dependent inhibitory effects of the peptides were observed for all peptides. Therefore, peptides targeting h31 of 16S rRNA have been identified and could be used as future drug molecules after refinement by peptidomimetics.
General Procedures for Examples 20-22
HPLC purification methods. The crude peptides required HPLC purification prior to binding studies. This step eliminated salt as well as other contaminants, such as failed sequences, organic reagents, etc., which may otherwise interfere with the binding studies. Purification was performed on a Luna® (Phenomenex) C18 reverse-phase column (250×10 mm) with water (0.05% TFA) as the mobile phase A and acetonitrile (0.05% TFA) as the mobile phase B at a flow rate of 5 μL/min. As a starting point, the lyophilized peptide was dissolved in water to form a 8-10 mg/ml solution, and a portion of it was then subjected to a test run at a gradient from 90% to 40% mobile phase A over a period of one hour. The subsequent method was then optimized based on the gradient at which the peptide was eluted in the test run. For the bulk purification, the lyophilized peptide was dissolved in water to give a 50-100 mg/mL solution, depending on the peptide solubility. The relevant fraction was collected and lyophilized to obtain the pure peptide. The HPLC traces corresponding to crude and purified peptides are given in the Appendix 5.
MALDI-TOF mass spectrometric methods. The synthetic peptides were characterized by MALDI-TOF mass spectrometry. A saturated matrix was made by dissolving 10 mg of α-cyano-4-hydroxycinnamic acid (α-cyano CHCA: Sigma-Aldrich®) in 1 mL of 50% acetonitrile in 0.05% TFA solution. This solution, in general, can be used for a long period of time (˜one year). The sample can be prepared by dissolving the purified peptide in 25% acetonitrile to give a 3-5 mg/mL solution. First, 10 μL from the saturated matrix was transferred to a small tube. To this, 1-10 μL of sample was added depending on its concentration and vortexed. Then, 2 μL from the resulting mixture was spotted onto the MALDI plate. Once the liquid was evaporated, the sample was used for the analysis.
RNA sample preparation. The RNA samples (ECh31WT) used in this study were chemically synthesized and purified as described in Chapter 4, Section 4.5.1. Three different versions of the ECh31 WT construct were employed for the binding experiments.
For circular dichroism experiments, h31 RNA was directly used without further processing or labeling. For the fluorescence experiments, the ECh31WT construct was 5′ labeled with fluorescein as described in Chapter 3, Section 3.5.2. For the SPR kinetic experiments, the ECh31WT construct was 5′ labeled with biotin as described in Chapter 3, Section 3.6.2.
Quantification of peptides. The concentration of the peptide sequences containing tryptophan or tyrosine was calculated based on the molar extinction coefficients (ε280) of these residues (δTrp=5560 and εTyr=1200 AU/mmole/mL).22 Since the extinction coefficients of chromophores in a given peptide sequence are additive, the overall molar extinction coefficient (e) of the peptide depends on the types and number of chromophores. Therefore, the milligrams (mg) of peptide in one milliliter (mL) of solution is given by the equation (A280×MW×DF)/ε, where A280 is the absorbance of the peptide, MW is the molecular weight of the peptide, DF is the dilution factor, and E is the total molar extinction coefficient of the peptide. For example, if the peptide has two tryptophan residues and one tyrosine residue, then the value ε is given by [(2×5560)+(1×1200)].
The concentration of GFP-fused peptides were determined by using a Micro BCA protein assay kit (Pierce™).23 This method of detection is based on the reduction of Cu2+ by protein in an alkaline medium, a strategy similar to the biuret assay.24 Then, the reduced Cu+ is colorimetrically detected by bicinchoninic acid (BCA).25
Circular dichroism (CD) studies. All CD measurements were done on a Chirascan™ circular dichroism spectrophotometer at 25° C. using a 1 cm pathlength quartz CD cuvette.
Structural characterization of peptides by CD. The peptides were dissolved in 10 mM HEPES-KOH, 100 mM KCl, 1 mM MgCl2, 0.5 mM EDTA, and 0.01% Triton-X-100 at pH 7.5 to obtain a 0.5 mg/mL solution. The spectra were obtained by scanning in the range of 180 nm to 250 nm.
Binding studies with CD. The titration was performed by adding increasing concentrations of peptide (10-80 μM) to 1 mL of 0.5 μM ECh31WT RNA in 10 mM sodium phoshate, 100 mM NaCl, 0.1 mM Na2EDTA at pH 7, and incubated for 2 min for each concentration point followed by spectrum scanning. Prior to titration, the RNA was renatured as described in Chapter 3, Section 3.2.2. RNA-peptide binding was determined by observing CD changes at 270 nm upon addition of peptide to the sample. The CD at 270 nm was converted to a fraction bound ratio and the dissociation constant (KD) of RNA-peptide binding was determined by curve fitting using the Kaleidagraph™ 3.0 program, as described in Chapter 3, Section 3.2.4.
Fluorescence methods. Fluorescence measurements were taken on a RF-5301PC spectrofluorometer (Shimadzu) at 25° C. using a 1 cm path-length quartz fluorometer cell. The emission spectra were acquired by scanning between 500 and 600 nm with an excitation wavelength of 494 nm, slit widths of 3 nm for excitation and emission. The fluorescent titrations were performed by adding increasing concentrations of peptide (5-150 μM) to 350 μl of 0.5 μM 5′-fluorescein-labeled helix 31 RNA in HEPES buffer (10 mM HEPES, 50 mM NaCl, 1 mM Na2EDTA at pH 7.5) and incubated for 2 min for each concentration point followed by spectrum scanning. Prior to titration, the RNA was renatured as described in Chapter 3, Section 3.5.2. RNA-peptide binding was determined by quenching of the fluorescence intensity upon addition of peptide to the sample. The fluorescence intensity at 523 nm was converted to a fraction bound ratio and the dissociation constant (KD) of RNA-peptide binding was determined by curve fitting using the Kaleidagraph™ 3.0 program, as described in Chapter 3, Section 3.5.3
SPR methods. All immobilization and subsequent binding studies were performed using a BIAcore 2000 instrument set at a temperature of 25° C. Standard dextran surface BIAcore sensorchips (Sensor chip CM5) were purchased from BIAcore. Standard desorb and sanitize routines were performed according to the BIAcore guidelines before docking a new CM5 sensor chip. All buffers were filtered through sterile 0.2 μm nylon membranes (Millipore™) under vacuum. Before derivatizing the flow cells with streptavidin, the CM5 sensor chip was pre-conditioned using three successive 10 μl injections of chip-preparation solution (10 mM NaOH, 500 mM NaCl) at 100 μl/min, followed by a normalization routine using BIAnormalizing solution (40% glycerol). Streptavidin derivatization was performed as described in Chapter 3. Prior to immobilization, the solution of biotinylated RNA in HBS-EP buffer (10 mM HEPES, 3 mM EDTA, 150 mM NaCl, 0.005% P20 at pH 7.4) was renatured by heating to 90° C. for 2 min followed by placing on ice. Flow cells were functionalized by injecting 30 μl of RNA at a time using the MANUAL INJECT command at a flow rate of 10 μl/min, until the desired immobilization level is reached. One of the flow cells was used to immobilize RNA (typically FC4), while another one adjacent to it (FC3) remained unmodified to serve as a blank-control for matrix effects. Levels of RNA captured were calculated by subtracting response units after injection from response units before injection for each flow cell. After RNA immobilization, FC3 and FC4 were blocked with 100 μL of 1 mg/mL biotin at 5 μL/min.
Peptide samples were prepared by serial dilutions from stock solutions into micro-centrifuge tubes. Dilutions are made by the same running buffer to avoid buffer mismatches. All procedures for binding were automated, as optimized methods using repetitive cycles of sample injection and regeneration. Typically, running buffer (10 mM Tris.HCl, 150 mM NaCl, 10 mM MgCl2, 1 mM DTT, 0.005% (v/v) P20 at pH 7.5) was injected for ˜30 min prior to experiment to establish a stable baseline value. Peptide solutions (200 μL) were injected at a kinetic flow rate (50 μL/min), using the KINJECT command. All peptide samples were injected from 7 mm plastic vials (BIAcore) that were capped with pierceable plastic-crimp-caps to minimize carry-over and sample evaporation. Samples were injected in order of increasing concentration. The surface was regenerated using 150 μL of 500 mM NaCl solution. The data were fit to a 1:1 binding Langmuir model using BIAevaluation 3.0.
Fmoc SPPS of Phage-Display Selected Peptides 7-Mer Peptides
Phage display is a biological system that facilitates the cloning and rapid selection of peptides from large combinatorial libraries.1, 17 The phage display library is a large, heterogeneous mixture of phage clones, each carrying a different foreign DNA insert, and therefore displaying a different peptide on the surface.2 An in vitro selection process called biopanning allows rapid identification of peptide ligands from this library. Biopanning was carried out by incubating the phage peptide library with the immobilized target (in this case the above-mentioned helix 31 wild-type construct), removing the unbound phage and eluting the target-bound phage. The eluted phage were amplified in cells to obtain a large crop of progeny phage, and these were then subjected to additional binding/amplification cycles to enrich the pool with the best binders.3 This phage-display procedure was carried out by Tek Lamichhane, in collaboration with the Cunningham laboratory.
In order to accomplish the above strategy, we constructed the wild-type E. coli h31 with its 5′ end biotinylated (Chapter 3). This step allowed the hairpin RNA to be immobilized onto a streptavidin-coated plate. Counterselection of ligands that can bind preferably to E. coli h31 over the h31 of H. sapiens has allowed us to come up with lead peptides as potential new bacterial anti-infectives (Table 13). The selected peptides were chemically synthesized or cloned so that they could be studied further. The chemical structures of the five peptides are shown in FIG. 49.
Individual peptides based on the sequence from phage display were prepared so that they can be further characterized for their affinities by biophysical techniques. During the screening process, the C-termini of peptides are not free. The peptides were displayed with the free N-termini exposed to the environment and the C-termini linked to the minor coat protein (P3) of M13 phage through a short spacer forming an amide bond. Therefore, the peptides were chemically synthesized on Rink Amide AM resin and obtained in their amidated forms as shown in
General procedure for the Fmoc 7-mer SPPS. All syntheses utilized Rink amide resin (Novabiochem®) preloaded with a 4-(2′,4′-dimethoxyphenyl-Fmoc-aminomethyl)-phenoxyacetamido-norleucylaminomethyl linker. This resin has a theoretical substitution level of 0.68 mmol/g. Generally, 250 mg of resin was used for each synthesis. Therefore, 0.17 (0.68×0.25) mmol of theoretical sites are available for coupling. First, 250 mg of resin was loaded into the peptide synthesis reaction vessel mounted on a wrist-action shaker. The initial suspension and swelling of the resin (45 min) took place with shaking using dichloromethane (DCM) followed by washing with dimethyl formamide (DMF). The procedure consisted of iterative deprotection, coupling, and washing steps. Fmoc deprotection was accomplished by treatment with piperidine-DMF (25% (v/v); 10× the resin volume) for 10 min with shaking, and a repeat with fresh deprotection solvent for 10 min, followed by DMF (5 times with 10× the resin volume) and DCM (5 times with 10× the resin volume) washing. Sequential coupling of residues involved mixing of Fmoc amino acid (3×0.68×0.25 mmol), DIC (4×0.68×0.25 mmol), HOBt (6×0.68×0.25 mmol), and DMF (5× the resin volume) with gentle shaking for 2 h. The side-chain protected Fmoc amino-acids were purchased from Novabiochem® (Appendix 3 and 4). The Kaiser test was used to confirm complete coupling, as indicated by a negative result; if the coupling was incomplete, additional DIC (4×0.68×0.25 mmol) was added and the vessel was shaken for an additional 2 h. If the coupling was complete, then the solution was drawn off, and the resin was washed with DMF (10× the resin volume). Coupling and deprotection steps were repeated for each added residue, with intervening washing steps (DMF, 10× the resin volume). After the final Fmoc deprotection, the resin was washed with DCM, DMF, ethyl ether, and acetone (twice each, 10× the resin volume). Finally, resin cleavage solution [5× the resin volume, TFA/TIS/thioanisole/anisole, 92:4:2:2 (v/v)] was added with shaking for 2 h. The solution was collected and separated equally into two 50 mL Falcon™ tubes, followed by addition of ethyl ether (−80° C.) to reach 80% of the total tube capacity. The solution was mixed, and the peptide precipitate formed immediately. After centrifugation (8 min at 6000 rpm), the supernatant was decanted, fresh ether was added, and the pelleted peptide was mixed prior to another round of centrifugation (repeated three additional times). Finally, the peptide was dissolved in distilled water (5-10 mL), frozen, and lyophilized for 24 to 48 h until a white powder was obtained.
As mentioned, the Kaiser test was used for the qualitative determination of coupling and deblocking. The Kaiser-test solutions contained the following components: Solution A—ninhydrin in ethanol (5% w/v), Solution B—phenol in ethanol (4:1, w/v), and Solution C—potassium cyanide in pyridine (2% v/v from a 1 mmol/L aqueous solution). The test was performed by adding 4 drops of solution A, 2 drops of solution B, and 2 drops of solution C to a tiny amount (<0.5 mg) of pre-washed resin contained in a small test tube. The test tube was heated to 100° C. for ˜2 minutes. A blue color in the beads was considered as a positive result, indicative of an incomplete coupling reaction.
TABLE 13
The round-4 sequences obtained after biopanning ECH31WT
RNA against a 7-mer phage library are summarized.
Peptide (sequence)
Frequency
14 (TLWDLIP)
5
15 (CVRPFAL)
5
16 (FVRPFPL)
6
17 (TYLPWPA)
5
18 (DIRTQRE)
4
Characterization of Peptides
The chemically synthesized peptides were purified by semi-preparative reverse-phase HPLC. Subsequently, the peptides were characterized using MALDI-TOF mass spectrometry and circular dichroism spectroscopy.
MALDI-TOF mass spectrometry. The peptide sequences were confirmed by checking for the correct molecular weights as shown in
Circular dichroism studies. In order to gain some information about the peptide behavior in solution, we investigated the peptide conformation by circular dichroism (CD) spectroscopy. The CD spectra were acquired in 10 mM HEPES-KOH, 100 mM KCl, 1 mM MgCl2, 0.5 mM EDTA, and 0.01% Triton-X-100 at pH 7.5 (
The data indicate the formation of α-helices by 14 (TLWDLIP (SEQ ID NO: 3)) and 17 (TYLPWPA (SEQ ID NO: 2)); where as the other three peptides appear to have random coil or other undefined structures. The presence of proline in many of the sequences has made the peptides behave more like polyproline type structures.
Determination of the Affinity of Phage-Display-Selected Peptides for h31
Once the peptides were synthesized, our goal was to find a suitable biophysical method to characterize the peptide-RNA interactions. These studies involved determination of binding affinities (equilibrium constants (Kd)) of peptides with the E. coli helix 31 hairpin RNA. Fluorescence, circular dichroism, and surface plasmon resonance (SPR) methods were employed to obtain Kd values for selected peptide-RNA interactions. Primarily, experiments were carried out with 17 (TYLPWPA (SEQ ID NO: 2)), because preliminary experiments with this peptide gave the most promising results.
Fluorescence titration assay. Helix 31 RNA was 5′-labeled with fluorescein (as described in Chapter 3) to monitor conformational changes in helix 31 upon binding of the peptide. A sample containing 0.5 μM of helix 31 was titrated with increasing concentrations of 17 (TYLPWPA (SEQ ID NO: 2)) (0-150 μM) in 10 mM HEPES, 50 mM NaCl, 1 mM Na2EDTA at pH 7.5. In this experiment, the fluorescence intensity decreased upon increases in the peptide concentration (
Hyperbolic curve fitting gave an apparent KD value of 27±4 μM (R2=0.97) and the Hill plot analysis indicated a single binding site (n=1.1) on the h31 target RNA (
Circular dichroism studies. CD was employed to assess the conformational changes in helix 31 upon binding of the peptide. A sample containing 0.5 μM helix 31 was titrated with increasing concentrations of 17 (0-80 μM) to obtain the spectra as shown in
The decrease in RNA CD signal upon increasing the peptide concentration implies a decrease in the helicity of the hairpin RNA. Interestingly, this may be due a destabilization of the hairpin RNA upon peptide binding. Further studies are underway (in collaboration with the SantaLucia group) to verify this effect by NMR spectroscopy.
SPR spectroscopic analysis. Helix 31 RNA was labeled with biotin (as described in Chapter 3) to determine the kinetics of peptide binding by SPR. Initial experiments performed with peptide 17 (TYLPWPA (SEQ ID NO: 2)) as the analyte gave negligible responses due to binding. In order to enhance the signal-to-noise ratio, a GFP-protein-fused peptide (17 (TYLPWPA)-GFP (“TYLPWPA” disclosed as SEQ ID NO: 2)) was used as the analyte (GFP, green fluorescent protein). The fusion protein was obtained by cloning the DNA sequence corresponding to 7-mer peptide sequence with the N-terminus of the GFP gene. The tobacco etch virus (TEV) protease-recognizing sequence was also cloned into the same construct, up field of the peptide gene sequence. Then, the protein was expressedin bacteria. Upon expression, TEV protease enzyme in the cell binds and cleaves the TEV—recognizing peptide sequence, generating the 7-mer peptide attached to the N-terminus of the GFP. This cloning procedure was performed by Tek Lamichhane in collaboration with the Cunningham lab.
Due to its larger size, a peptide fused with GFP has a greater change in refractive index on the SPR surface, hence generating a significant signal response upon binding to RNA. Biotinylated helix 31 RNA was immobilized onto a streptavidin-coated CM5 chip and differing concentrations of 17 (TYLPWPA)-GFP (“TYLPWPA” disclosed as SEQ ID NO: 2) were injected as the analyte. Control experiments were performed by varying the salt concentrations, detergent levels, pH conditions, and flow rates, since these factors could affect the peptide-RNA complex formation in solution. Finally, the apparent dissociation constants were determined under optimized conditions.
A) Salt Concentration Effects
Preliminary experiments were performed with varying salt concentrations (50 to 250 mM NaCl) to determine the salt effects on 17 (TYLPWPA)-GFP (“TYLPWPA” disclosed as SEQ ID NO: 2) binding to h31 RNA. Salt concentration is an important factor that could affect the RNA-peptide interactions. The buffer used for these experiments contained 10 mM Tris.HCl at pH 7.5, 10 mM MgCl2, 1 mM DTT, 0.005% (v/v) surfactant P20, and varying concentrations of NaCl. The results obtained by injecting 50 μM concentration of 17 (TYLPWPA)-GFP (“TYLPWPA” disclosed as SEQ ID NO: 2) are shown in
The results suggest that there is an enhanced binding of the peptide to the RNA at lower salt concentrations (<150 mM NaCl), possibly due to increased non-specific interactions under such conditions. That is evident from the fast association as well as the very slow dissociation of the peptide (
B) Effects of Detergent
Another common way to avoid non-specific binding in SPR is the addition of detergents. These detergents also prevent aggregation of proteins at high concentrations. Varying amounts of polysorbate 20 (P20) were added to the SPR buffer (10 mM Tris.HCl at pH 7.5, 150 mM NaCl, 10 mM MgCl2, 1 mM DTT) to observe any effects from the detergents. The results obtained by injecting 50 μM concentration of 17 (TYLPWPA)-GFP (“TYLPWPA” disclosed as SEQ ID NO: 2) are shown in
The results indicate a significant decrease in signal upon increasing the detergent concentration, despite the fact that higher amounts of detergent are known to decrease the non-specific binding of the proteins.19 Therefore, the level of P20 was maintained at 0.005% (V/V) in the subsequent experiments.
C) Effects of Buffer pH
The pI of 17 (TYLPWPA)-GFP (“TYLPWPA” disclosed as SEQ ID NO: 2) is predicted to be 6.20 therefore, if the pH is <6.0 there will be a net positive charge on the protein. In order to observe the effects of buffer-pH on the peptide binding, a series of buffers with varying pH (5.6 to 7.5) were employed (
The sensorgrams at pH>6.0 showed no significant changes in the response units (RUs). Therefore, it was decided that pH 6.9 to 7.5 is an effective pH range within which the binding experiments could be performed. The above result also suggests that the interaction between 17 (TYLPWPA)-GFP (“TYLPWPA” disclosed as SEQ ID NO: 2) and h31 RNA may be governed by a dominant electrostatic component along with stacking, hydrogen bonding, or metal-mediated binding. Further investigations are necessary to determine these effects conclusively.
D) Effects of Flow Rate
The flow rate is considered as another important parameter that should be investigated in SPR analysis.21 The reason for this optimization is to eliminate any mass transfer issues during the binding experiments (discussed in Section 3.6.4). Sensorgrams were obtained at different flow rates (40, 50 and 60 μL/min) to determine a suitable flow rate at which the experiments can be performed (
The results in
From this point onwards, all the data reported on kinetic analyses of peptide binding to RNA were obtained in 10 mM Tris.HCl, 150 mM NaCl, 10 mM MgCl2, 1 mM DTT, 0.005% (v/v) P20 at pH 7.5 as the running buffer at a flow rate of 50 μL/min.
By making use of the information gained from the above control experiments, an optimized set of conditions were revealed to investigate the affinity of the peptides to helix 31 RNA. In addition to the aforementioned general control experiments, several specific controls (such as injection time, dissociation time, regenerating salt concentration, etc.) were also performed with respect to each peptide that was employed. Based on the above information, a typical sensorgram that is observed in this study is shown in
Biotinylated helix 31 RNA was immobilized onto a streptavidin-coated CM5 chip and increasing concentrations of 17 (TYLPWPA)-GFP (0-100 μM) were injected in the KINJECT mode to obtain the data in
TABLE 14
Affinity data obtained through SPR kinetic analysis of
a 1:1 interaction between h31 and 17 (TYLPWPA)-GFP.
17 (TYLPWPA)-GFP
ka (M−1s−1)
150
SE
2.0
kd (s−1)
4.2 × 10−3
SE
3.8 × 10−5
KD (μM)
28 ± 1
χ2
0.5
Consistent KD values were obtained for the interaction of 17 (TYLPWPA) with helix 31 from fluorescence, CD, and SPR experiments as summarized in Table 15. The results reveal that the binding of 17 (TYLPWPA) to helix 31 has not been affected by the presence of GFP. From these experiments, peptide 17 (TYLPWPA) is found to have moderate affinity for helix 31.
TABLE 15
The binding affinity of 17 (TYLPWPA) towards h31 RNA
obtained through different biophysical techniques.
Technique
Observed KD (μM)
fluorescence
27 ± 4
circular dichroism
28 ± 10
SPR
28 ± 1
In our next attempt, we extended the SPR kinetic analysis to two other peptides discovered from the phage display technology, namely 14 (TLWDLIP)-GFP and 15 (CVRPFAL)-GFP. Biotinylated helix 31 RNA was immobilized onto a streptavidin-coated CM5 chip and increasing concentrations of 14 (TLWDLIP)-GFP (0-1 μM) and 15 (CVRPFAL)-GFP (0-1 μM) were injected in the KINJECT mode to obtain the data shown in
TABLE 16
Affinity data obtained through SPR kinetic analysis
of 14 (TLWDLIP)-GFP and 15 (CVRPFAL)-GFP are shown.
14 (TLWDLIP)-GFP
15 (CVRPFAL)-GFP
ka (M−1s−1)
9.3 × 103
1.2 × 104
SE
156
112
kd (s−1)
3.1 × 10−3
2.6 × 10−3
SE
3.3 × 10−5
1.8 × 10−5
KD (nM)
330 ± 7
230 ± 3
χ2
2.1
1.4
G) SPR Kinetic Analysis of GFP-Affinity Towards Helix 31 RNA
In order to improve the signal-to-noise ratio in the SPR studies, the peptides were cloned to GFP by molecular cloning techniques (performed by Tek Lamichhane in collaboration with the Cunningham lab) as mentioned earlier. Adequate control experiments were also performed to minimize the non-specific binding of GFP to helix 31. Despite these efforts, a reasonable non-specific interaction was still observed for GFP alone. Therefore, it was necessary to evaluate the affinity of GFP towards helix 31. A control kinetic experiment was performed with free GFP. Biotinylated helix 31 RNA was immobilized onto a streptavidin-coated CM5 chip and increasing concentrations of GFP (0-100 μM) were injected in the KINJECT mode to obtain the data shown in
TABLE 17
Affinity data obtained through SPR kinetic analysis
of a 1:1 interaction between h31 and GFP protein.
GFP
ka (M−1s−1)
222
SE
3.1
kd (s−1)
4.4 × 10−3
SE
3.6 × 10−5
KD (μM)
20 ± 1
χ2
1.3
The Specificity of the Phage display Peptides for ECh31WT RNA—Preliminary Studies
The GFP fused peptides were tested for their specificity to ECh31WT RNA by a SPR analysis. The biotinylated RNA constructs were attached to the SA chip in the following order.
The sensorgrams were acquired in the 2-1, 3-1, 4-1 detection mode.
The affinities for ECh31WT RNA (Fc 3-1) were compared with ECh31UNMOD (Fc 4-1) (
Additionally, the affinities for HSh31ECstem RNA (Fc 2-1) were studied (
The affinities for TAR RNA (Fc 2-1) were compared with ECh31WT (Fc 4-3). The RNA constructs were immobilized in the following order:
All of the references including, without limitation, U.S. patents, U.S. patent application publications, published international applications and journal articles cited herein are hereby incorporated by reference.
Those skilled in the art will recognize, or be able to ascertain using no more than routine experimentation, many equivalents to the specific embodiments of the invention described herein. Such equivalents are intended to be encompassed by the following claims.
Cunningham, Philip R., Chow, Christine Sharon, Abeydeera, Nuwan Dinuka, Lamichhane, Tek Narayan
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